METHODS FOR MAKING ARRAYS FOR HIGH THROUGHPUT PROTEOMICS
20180016299 ยท 2018-01-18
Inventors
Cpc classification
B01J2219/00605
PERFORMING OPERATIONS; TRANSPORTING
C12N2710/24134
CHEMISTRY; METALLURGY
C12N2795/10222
CHEMISTRY; METALLURGY
Y02A50/30
GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
C07K14/00
CHEMISTRY; METALLURGY
C12N15/1034
CHEMISTRY; METALLURGY
C07K1/1077
CHEMISTRY; METALLURGY
C12N15/1086
CHEMISTRY; METALLURGY
C12N15/1093
CHEMISTRY; METALLURGY
A61K39/015
HUMAN NECESSITIES
C12N2800/70
CHEMISTRY; METALLURGY
C12N2710/24143
CHEMISTRY; METALLURGY
International classification
C07K1/107
CHEMISTRY; METALLURGY
A61K39/015
HUMAN NECESSITIES
Abstract
Methods to obtain expression systems and proteins in a high-throughput protocol by utilizing mixtures of cells cultured from those transformed with a desired nucleotide sequence permit rapid production of protein for use in arrays to assess activity. In one embodiment, the proteins (or peptides) in the array are assessed for their immunological activity with regard to an infectious agent.
Claims
1 to 67. (canceled)
68. A method of making an array, wherein the array comprises a plurality of different, individual and non-pure recombinant proteins and/or peptides of at least one pathogen, infectious agent or prokaryote having a known genome affixed on a plurality of distinct, individually addressable locations on a surface of a substrate, a plate or chip to produce an array of distinct, individually addressable locations, wherein the plurality of recombinant proteins and/or peptides comprises at least about 100 proteins and/or peptides and represents at least about 50% of the genome of the pathogen or infectious agent, or if the known genome is the genome of an infectious agent or the genome of the prokaryote, the plurality of different, individual and non-pure recombinant proteins and/or peptides comprises at least about 10% of the proteins and peptides expressed by the pathogen, infectious agent or prokaryote having a known genome, wherein the method of making the array comprises: (a) providing a plurality of linearized expression vectors; (b) providing a plurality of amplification primers comprising sequences capable of amplifying a desired number of open reading frame (ORF) coding sequences encoding the plurality of recombinant proteins and/or peptides expressed by the pathogen, infectious agent or prokaryote having a known genome, wherein each of the plurality of amplification primers contains both a sequence complementary to an end portion of one of the desired number of the ORF coding sequences and an adapter being homologous to a sequence provided on a linearized expression vector or on the plurality of linearized expression vectors, and using an amplification technique to amplify individually a desired number of open reading frames (ORF) coding sequences to obtain a plurality of individually amplified segments, (c) providing a recombinase-containing host cell; (d) co-transfecting into the recombinase-containing host cell the plurality of amplified products and the plurality of linearized expression vectors; (e) culturing the co-transfected host cell for sufficient time on or in a suitable medium to allow homologous recombination of the plurality of amplified products and the plurality of linearized expression vectors in vivo, wherein the plurality of linearized expression vectors and the plurality of amplified products are ligated by homologous recombination in vivo in the cells to generate a plurality of ligated expression vectors; (f) extracting or harvesting from the host cell the plurality of ligated expression vectors; (g) translating the plurality of ligated expression vectors in: (1) a cellular derived system, which is a cell-free in vitro translation system, to obtain a peptide- and/or protein-containing mixture, or (2) a suitable host cell in vivo, wherein the translation generates a peptide and/or protein containing or comprising the peptide- and/or protein-containing mixture, and (g) spotting or placing the peptide- and/or protein-containing mixture directly onto a solid support to generate the array of different, individual and non-pure recombinant proteins and/or peptides of at least one pathogen, infectious agent or prokaryote having a known genome.
69. The method of claim 68, wherein the plurality of different, individual and non-pure recombinant proteins and/or peptides represents at least about 70% of the genome of the pathogen or infectious agent.
70. The method of claim 68, wherein if the known genome is the genome of an infectious agent or the genome of any prokaryote, the plurality of different, individual and non-pure recombinant proteins and/or peptides represents at least about 20% of the proteins and peptides expressed by the pathogen or prokaryote having a known genome.
71. The method of claim 68, wherein the pathogen, infectious agent or prokaryote is selected from the group consisting of a Vaccinia virus, a human Papillomavirus, a West Nile virus, Francisella tularensis, Burkholderia pseudomallei, Plasmodium falciparum, and Mycobacterium tuberculosis.
72. The method of claim 68, wherein a portion of the cell-free in vitro translation system comprises a supernatant of the cell-free expression extract.
73. The method of claim 68, wherein the expression vector is a plasmid.
74. The method of claim 68, wherein the cell-free in vitro translation system is a prokaryotic or a eukaryotic cell-free in vitro translation system.
75. The method of claim 74, wherein the prokaryotic cell-free in vitro translation system is a bacterial cell-free in vitro translation system
76. The method of claim 74, wherein the eukaryotic cell-free in vitro translation system is a mammalian, a plant, an insect or a human reticulocyte cell-free in vitro translation system.
77. The method of claim 68, wherein the ratio of expression vector to cells in the transfection reaction is adjusted to be at most 100 ng/million cells, or 1 to 10 ng /million cells.
78. The method of claim 68, wherein the solid support is a microtiter plate, a chip or a nitrocellulose substrate.
79. The method of claim 68, wherein the pathogen is selected from the group consisting of a Vaccinia virus, human papilloma virus, West Nile virus, Francisella tularensis, Burkholderia pseudomallei, Plasmodium falciparum, and Mycobacterium tuberculosis.
80. The method of claim 70, wherein if the known genome is the genome of an infectious agent or the genome of any prokaryote, the plurality of different, individual and non-pure recombinant proteins and/or peptides represents at least 50% of the proteins and peptides expressed by the pathogen or prokaryote having a known genome.
81. The array of claim 80, wherein if the known genome is the genome of an infectious agent or the genome of any prokaryote, the plurality of different, individual and non-pure recombinant proteins and/or peptides represents at least 75% of the proteins and peptides expressed by the pathogen or prokaryote having a known genome.
82. The array of claim 81, wherein if the known genome is the genome of an infectious agent or the genome of any prokaryote, the plurality of different, individual and non-pure recombinant proteins and/or peptides represents at least 90% of the proteins and peptides expressed by the pathogen or prokaryote having a known genome.
83. The method of claim 68, wherein the amplification technique comprises a polymerase chain reaction (PCR).
84. The method of claim 68, wherein the translating of the plurality of ligated expression vectors obtained in a cellular derived system is in a cell-free in vitro translation system.
Description
BRIEF DESCRIPTION OF THE DRAWINGS
[0039]
[0040]
[0041]
[0042]
[0043]
[0044]
[0045]
[0046]
[0047]
[0048]
[0049]
[0050]
[0051]
[0052]
[0053]
MODES OF CARRYING OUT THE INVENTION
[0054] One embodiment of the invention provides a high throughput method to obtain an array of proteins and/or peptides representative of those encoded in the genome of an infectious agent so that the arrays can be tested for their ability to effect a humoral and/or cellular immune response. The method for preparing the proteins in the array is applicable to the preparation of proteins in general, from any source. In particular, the high throughput advantages inherent in the method are applicable in providing a repertoire of proteins and peptides from infectious agents. The method could also be used for providing a multiplicity of proteins and/or peptides encoded by any nucleic acid of known sequence so that individual
[0055] amplified portions or inserts may be provided to plasmids replicable in recombinase-containing microorganisms. The invention method for preparation of such proteins differs from those employed previously in that it employs DNA extracted from mixtures of microorganisms obtained by culturing the components of a transformation mixture rather than isolating individual clones. This is advantageous as isolation of clones often results in obtention of a mutant rather than the desired native form of the protein. Further, the invention method may employ, in the screening phase, unpurified forms of the proteins encoded by and expressed from vectors obtained from these mixtures. As a result, the present method greatly simplifies automation of the overall process and adoption of high-throughput processing.
[0056] Using the method of the invention, it has been possible to identify particular proteins from vaccinia that will be potent vaccines. This is of considerable significance as the use of attenuated virus is sometimes associated with unwanted side effects. It would be preferable to utilize a single protein or defined mixture of proteins, rather than the complex infectious agent in attenuated form. This is done currently, for example, using hepatitis B surface antigen.
[0057] The invention method is applicable, as stated above, to nucleic acids that encode a multiplicity of proteins and peptides in general where the relevant nucleotide sequence is known, so that appropriate primers can be employed to effect the amplification of the desired insert. As described in, for example, US2003/0082579 and US2003/0044820, both incorporated herein by reference, the designed primers may include adapter sequences that provide for the desired homologous recombination with a linearized vector. The extended primers themselves and/or the linearized vector may then provide appropriate control sequences, such as promoters and terminators to effect expression as well as tags such as histidine tags, FLAG tags, and the like, to permit strengthened binding to an appropriate solid surface or, if desired, purification of the expressed protein. Commonly, the linearized vector is also amplified by PCR, rather than using the more traditional method of vector digestion, which can result in vectors which fail to contain inserts.
[0058] In the overall method of the invention, a nucleic acid molecule, such as an infectious agent genome, that encodes a multiplicity of proteins or peptides and whose nucleotide sequence is known, is used as the substrate. Each segment that encodes a protein or peptide of interest is individually (i.e., in an individual reaction mixture) amplified using PCR or other amplification techniques employing primers that contain both a sequence complementary to an end portion of the coding sequence and an adapter that may encode a tag and/or a sequence that controls expression, but which, in any event, is homologous to sequences provided on a linearized plasmid. The individually amplified segment and linearized plasmid are then cotransfected into a recombinase-containing microorganism to permit recombination in vivo. The recombinase-containing organisms may be, for example, yeast or may be a chemically competent E. coli (or, less desirably, an electroporation competent E. coli). Suitable chemically competent E. coli include the strains JC8679, TB1, DH5a, HB101, JM101, JM109 and LE392. Saccharomyces are particularly effective with regard to recombinase-containing yeast.
[0059] The ratio of DNA to cells in the transfection reaction may be as high as 100 ng/million cells; however, ratios of as low as 1-10 ng, 5-10 ng, 1-5 ng or 1-3 ng/million cells may also be used. It is often desirable to provide the linearized plasmid and the desired nucleotide sequence in about a 1:1 molar ratio, though ratios from 5:1 to 10:1 to 100:1 may be used, and ratios of 1:5 to 1:10 to 1:100 may also be used.
[0060] The cells thus treated with the amplified insert and the amplified linearized vector are cultured on suitable medium, often overnight. The resultant is a mixture of cells, most of which will contain the desired recombined vector having the anlplified segment of the desired nucleotide sequence inserted in the correct orientation. (Directionality is ensured by the design of the primers to match the homologous portions of the linearized plasmid.) Rather than isolating individual colonies, which risks loss of the desired insert in favor of, for example, a mutant, the cells are harvested from the culture and extracted directly to obtain the plasmid DNA. The plasmid mixture thus obtained is then subjected to transcription/translation either by transfecting the DNA into suitable host cells, or commonly for the purposes of high throughput, in an in vitro translation system. Such in vitro translation systems are commercially available, and methods for their use are well known to those of skill in the art. The resulting protein or peptide can then be directly spotted onto a solid support, which support may be a portion of an array of proteins and peptides prepared on any suitable surface, such as the wells of a microtitre plate or segmented nitrocellulose. The protein may, if desired, be purified by methods known in the art, or by using a tag that was encoded into it from the primer or plasmid, or, alternatively, the transcription/translation mixture can be used directly without further purification of the protein to provide the protein or peptide to the solid support. Purified or substantially purified proteins produced by this method are one aspect of the invention. Those proteins or peptides may be naturally occurring peptides or modified versions comprising one or more additions such as an epitope tag as further described herein. Where the proteins are adhered to a support, the solid support may, itself, be supplied with a counterpart ligand to a tag on the protein or peptide.
[0061] In order to obtain an array of proteins, the foregoing sequence of steps is performed with respect to as many ORF's or portions thereof as desired. It may be advantageous to obtain only a relatively small number of proteins or peptides as members of the protein/peptide array if promising candidates are already known for whatever screen is to be performed on the array. However, a multiplicity of nucleotide sequences may be turned into proteins or peptides; as many as 50, 100, 500, 1,000 or more. If the genome of an infectious agent is used, for example, or the genome of any prokaryote, the array may include at least 10%, 20%, 50%, 75%, 90%, 95% or 100% of the proteins and peptides expressed. The resultant array may represent substantially the entire proteome of the organism, i.e. at least about 98% of the proteome or only a portion thereof, or may represent individual peptide portions of the proteins in the proteome, or a combination of full-length proteins and partial sequences.
[0062] In order to facilitate the preparation of an array of peptides or proteins, it may be advantageous to fuse the peptide or protein of interest with a short peptide tag, which is commonly 6 to 20 amino acids in length, that binds to a specific functional group. Such binding tags can then be used for purification of the protein or to affix the protein to a test surface, or to detect the presence of the protein. Such binding tags consisting of short sequences of amino acids are well known and are commonly referred to as epitope tags. For example, a hemagglutinin (HA) epitope tag (such as the human influenza hemagglutinin protein, YPYDVPDYA) or a c-Myc epitope tag (a 10 amino acid segment of the human protooncogene myc, EQKLISEEDL) may be fused to the peptide or protein to be expressed by incorporating the appropriate nucleotide sequence into the adapter used to insert the genomic nucleic acid into an expression plasmid. Antibodies to the c-Myc, HA, or other epitope tag may then be used to detect or localize the expressed peptide.
[0063] Similarly, a poly-histidine tag may serve as an epitope tag and may be incorporated into the expressed protein by proper design of the adapters used to insert the genomic nucleic acid into the vector used for expressing the protein. A poly-histidine epitope tag may contain 3 to 12 consecutive histidine residues, commonly 6-10 consecutive histidine residues. Such poly-histidine tag will specifically and tightly bind to a nickel surface; thus the expressed peptide or protein containing such a tag will bind tightly to a nickel bead, a nickel-coated surface, or an affinity column comprising nickel or a nickel salt or complex such as, for example, nickel nitrilotriacetic acid (Ni-NTA). An array of proteins or peptides containing poly-histidine tags can thus be produced in a 96-well format by coating each well with nickel or a nickel salt or complex, then placing a solution of each protein or peptide into such a nickel-coated well and allowing the protein to become affixed to the surface. Similarly, such proteins can be attached to a bead for convenient display by making beads of nickel or by plating beads of other material with nickel or a nickel salt or complex. In one embodiment, the proteins of a genome are tagged with a poly-his tag comprising at least 6 consecutive histidine residues and are allowed to adhere to 1 um nickel beads; these beads are then used to assay for immunological response by T-cells as described in Example 9, infra.
[0064] Where desired, it is also possible to attach two different tags: a nucleotide sequence coding for a first tag can be included near the 5 end of the nucleic acid inserted into the plasmid to attach a tag at the N-terminal of the expressed protein, and a nucleotide sequence coding for a second tag can be included near the 3 end of the nucleic acid inserted into the plasmid to attach a tag near the C-terminal end of the expressed protein. These tags could be the same, to insure recognition in case one terminus is buried and thus inaccessible; or they may be different, to enable two different capture or detection methods to be used. Other tags useful for detection, localization or purification may also be attached to the genomic protein as needed. Such tags include glutathione-S-transferase (GST), biotinylation signals, green fluorescent protein (GFP) and the like, each of which can be incorporated by methods well known in the art.
[0065] Once the desired peptides/proteins or array of peptides/proteins is obtained, it may be screened for any desired property or reactivity. One example of such use is screening for immunoactive peptides and proteins. The immunoactivity may be with respect to the humoral or the cellular system. In either case, a screening agent obtained from a subject that has been exposed to the infectious agent or some portions thereof is required. Optionally, the array of proteins or peptides may be screened against one or more immune components (serum, sputum, plasma, T-cells, etc.) from multiple subjects, each of which has been exposed to the infectious agent or some portion of it such as its envelope proteins or lysed cells, or one or more of its proteins. This permits determination of which antigens elicit immune responses in multiple subjects: those most commonly recognized are referred to as immunodominant antigens. A family of antigens may be useful in a serological diagnostic test or in a vaccine comprising several of these immunodominant antigens.
[0066] The methods of the invention can be applied to a variety of genomes, and are often usefully applied to the genomes of infectious agents, including viruses, fungi, bacteria, protozoa and the like as well as multicellular parasites such as flatworms, flukes, roundworms, and the like. By providing methods to quickly produce an array of proteins that represent most of all of the proteome of such an infectious agent, the invention makes it possible to quickly identify those genes and proteins most useful for the development of vaccines or diagnostic tests against a particular infectious agent.
[0067] Thus, as used herein, the term immunoactive refers to the ability of a protein or peptide to elicit an immune response, whether that response is humoral or cellular, or both. A humoral immune response is an adaptive protection mechanism that is characterized by the production of antibodies, while a cellular immune response is characterized by the production and/or activation of cells such as activated natural killer (NK) cells and cytotoxic T-lymphocytes (T-cells, or CTL). Similarly, antigen refers to such immunoactive proteins or peptides, regardless of the nature of the immune response elicited. Immunodominant antigen refers to an antigen that elicits an immune response in most or all subjects exposed to the antigen; such immunodominant antigens are most likely to provide effective vaccine components or elicitors of antibody production for use in passive immunization methods, and are therefore often especially useful as components of an immunologic composition and will also be useful in serological diagnostic tests..
[0068] T cells recognize peptide/MEC complexes on the surface of other cells. Such cells are often referred to as antigen presenting cells (APCs). Although effector cells can mediate their functions by recognizing such complexes on virtually any cell type, naive cells are most efficiently activated by a set of specialized APCs, the dendritic cells (DCs).
[0069] Array as used herein refers to a collection of materials systematically positioned on at least one test surface, including materials contained in wells or depressions formed on said surface, where the placement of the material is correlated to the identity of the material. An array generally contains at least about 10 materials so positioned, and often contains at least 100 or 200 or 500, or it may contain 1000 or more materials. It includes materials spotted onto a chip, plate, or nitrocellulose substrate, for example, and materials contained in the wells of 96-well and 384-well and similar plates, as long as the materials are retained in the location where they were placed, whether they are retained due to physical or chemical forces. An array may comprise multiple plates, chips or other surfaces. A microarray is a miniaturized array that may be designed to minimize reagent volumes, for example. While the arrays described herein are often arrays of antigenic peptides, the invention also includes arrays of antibodies that are selective for such antigenic peptides.
[0070] The antigens identified by the method of the invention may be peptides or proteins and are used to prepare immunologic compositions for protecting subjects against infection by the infectious agent or to generate monoclonal antibodies useful for providing passive immunization or for purification or detection of the antigens. Such immunologic compositions may be vaccines that induce a subject to produce an immune response such as the production of antibodies, or they may themselves be antibodies or active immunological materials that provide passive immunity. Anti-idiotypic antibodies or nucleic acids that generate them may be used in lieu of the antigens themselves. They may also be nucleic acid vaccines that generate one or more antigenic epitopes, wherein the nucleic acid can be taken up by the subject's own cells. They may be accompanied by functional elements such as promoters that effect production of the encoded antigenic protein or peptide, or may be naked DNA.
[0071] The invention also includes those peptides and antigens that are substantially homologous to those identified by the methods of the present invention, as well as immunologic compositions derived from such substantially homologous antigens. Thus it includes diagnostic tests or vaccines containing peptides or proteins that are substantially homologous to those peptides or proteins identified by the methods described herein; it includes antibodies specific for antigens that are substantially homologous to those antigens identified by the methods described herein; and it includes nucleic acids having nucleotide sequences encoding these substantially homologous peptides or proteins.
[0072] The term substantially homologous, when used herein with respect to a protein or peptide, means a protein or peptide corresponding to a reference protein or peptide, wherein the protein or peptide has substantially the same structure and function as the reference, for example, where only changes in amino acids sequence not affecting function occur. Thus, in the present application, the substantially homologous peptides and proteins are immunoactive and have similar structures to the reference. With regard to structure, the percentage of identity between the substantially homologous versus the reference protein or peptide is at least 65%, or at least 75%, or at least 85%, or at least 90%, or at least 95%, or at least 99%.
[0073] Alignment of protein sequences for identity comparison can be conducted by art known method. Useful methods for comparison of protein sequences include the local homology algorithm of Smith & Waterman, Adv. Appl. Math. 2: 482 (1981); the homology alignment algorithm of Needleman & Wunsch, J. Mol. Biol. 48: 443 (1970); the search for similarity method of Pearson & Lipman, Proc. Nat'l. Acad. Sci. USA 85: 2444 (1988); computerized implementations of these algorithms (GAP, BESTFIT, PASTA, and TFASTA in the Wisconsin Genetics Software Package, Genetics Computer Group, 575 Science Dr., Madison, Wis.); and visual inspection (see generally, Ausubel et al., infra).
[0074] An example of an algorithm that is suitable for determining percent sequence identity and sequence similarity is the BLAST algorithm, which is described in Altschul et al., J. Mol. Biol. 215: 403-410 (1990). Software for performing BLAST analyses is publicly available through the National Center for Biotechnology Information at the web site www.ncbi.nlm.nih.gov. This algorithm involves first identifying high scoring sequence pairs (HSPs) by identifying short words of length Win the query sequence, which either match or satisfy some positive-valued threshold score T when aligned with a word of the same length in a database sequence. T is referred to as the neighborhood word score threshold (Altschul et al., 1990). These initial neighborhood word hits act as seeds for initiating searches to find longer HSPs containing them. The word hits are then extended in both directions along each sequence for as far as the cumulative alignment score can be increased. Cumulative scores are calculated using, for nucleotide sequences, the parameters M (reward score for a pair of matching residues; always >0) and N (penalty score for mismatching residues; always <0). For amino acid sequences, a scoring matrix is used to calculate the cumulative score. Extension of the word hits in each direction are halted when the cumulative alignment score falls off by the quantity X from its maximum achieved value, the cumulative score goes to zero or below due to the accumulation of one or more negative-scoring residue alignments, or the end of either sequence is reached. The BLAST algorithm parameters W, T, and X determine the sensitivity and speed of the alignment. For amino acid sequences, the BLASTP program uses as defaults a wordlength (W) of 3, an expectation (E) of 10, and the BLOSUM62 scoring matrix (see Henikoff & Henikoff, Proc. Natl. Aca. Sci. USA (1989) 89: 10915).
[0075] Sequence alignments may also be performed using the Megalign program of the LASERGENE bioinformatics computing suite (DNASTAR Inc., Madison, Wis.). Multiple alignment of the sequences may be performed using the Clustal method of alignment (Higgins and Sharp (1989) CABIOS. 5:151-153) with the default parameters (GAP PENALTY=10, GAP LENGTH PENALTY=10). Default parameters for pairwise alignments using the Clustal method may be, for example, KTUPLE 1, GAP PENALTY=3, WINDOW=5 and DIAGONALS SAVED=5.
[0076] In the alternative, proteins or peptides are also considered substantially homologous herein when they are immunologically cross reactive. A variety of immunoassay formats may be used to select antibodies specifically immunoreactive with a particular protein or peptide. For example, solid-phase ELISA immunoassays, Western blots, or immunohistochemistry are routinely used to select monoclonal antibodies specifically immunoreactive with a protein. See Harlow and Lane (1988) Antibodies, A Laboratory Manual, Cold Spring Harbor Publications, New York Harlow and Lane), for a description of immunoassay formats and conditions that can be used to determine specific immunoreactivity. Typically a specific or selective reaction will be at least twice background signal or noise and more typically more than 10 to 100 times background.
[0077] One of ordinary skill in the art will recognize that individual substitutions, deletions or additions that alter, add or delete a single amino acid or a small percentage of amino acids (for example, less than about 5%, or for example, less than about 1%) in a sequence are conservatively modified variations, where the alterations result in the substitution of an amino acid with a chemically similar amino acid. Conservative substitution tables providing functionally similar amino acids are well known in the art. The following five groups each contain amino acids that are conservative substitutions for one another: Aliphatic: Glycine (G), Alanine (A), Valine (V), Leucine (L), Isoleucine (I); Aromatic: Phenylalanine (F), Tyrosine (Y), Tryptophan (W); Sulfur-containing: Methionine (M), Cysteine (C); Basic: Arginine (R), Lysine (K), Histidine (H); Acidic: Aspartic acid (D), Glutamic acid (E), Asparagine (N), Glutamine (Q). See also, Creighton (1984) Proteins, W.H. Freeman and Company. Conservatively modified variations of a described nucleic acid nucleotide sequence or polypeptide amino acid sequence is implicit in each described sequence.
[0078] One aspect of the present invention relates to nucleotide sequences that encode all or a substantial portion of the amino acid sequence encoding the proteins or substantial portions thereof identified herein. (One example of such proteins is H3L Western Reserve Strain, H3L Copenhagen Strain and H3L Variola Major Bangladesh Strain proteins.) A substantial portion of a protein comprises enough of the amino acid sequence to afford putative identification, either by manual evaluation of the sequence by one skilled in the art, or by computer-automated sequence comparison and identification using algorithms such as BLAST (Basic Local Alignment Search Tool; Altschul, S. F., et al., (1993) J. Mol. Bioi. 215:403-410). In general, a sequence of nine or more contiguous amino acids is necessary in order to putatively identify a protein as homologous to a known protein. Substantially homologous protein fragments may be identified by the percent identity of the amino acid sequences of the fragments compared to those proteins disclosed herein.
[0079] As noted in greater detail below, the immunogenic peptides can be prepared synthetically, such as by chemical synthesis or by recombinant DNA technology, or isolated from natural sources such as whole viruses or other infectious agents. Although the peptide will often be substantially free of other naturally occurring host cell proteins and fragments thereof, in some embodiments the peptides can be synthetically conjugated to native fragments or particles.
[0080] Peptides having the desired activity may be modified as necessary to provide certain desired attributes, e.g., improved pharmacological characteristics, while increasing or at least retaining substantially all of the antigenic activity of the unmodified peptide. For instance, the peptides may be subject to various changes, such as substitutions, either conservative or non-conservative, where such changes might provide for certain advantages in their use, such as improved MHC binding. The range of amino acid substitutions may also include using D-amino acids. Such modifications may be made using well known peptide synthesis procedures, as described in e.g., Merrifield, Science 232:341-347 (1986), Barany and Merrifield, The Peptides, Gross and Meienhofer, eds. (N.Y., Academic Press), pp. 1-284 (1979); and Stewart and Young, Solid Phase Peptide Synthesis, (Rockford, Ill., Pierce), 2d Ed. (1984), each of which is incorporated herein by reference.
[0081] The pharmaceutical compositions for therapeutic treatment are intended for parenteral, topical, oral or local administration. In some embodiments it may be desirable to include in the pharmaceutical compositions of the invention at least one component which primes CTL. Lipids have been identified as agents capable of priming CTL in vivo against viral antigens. For example, palmitic acid residues can be attached to the alpha and epsilon amino groups of a Lys residue and then linked, e.g., via one or more linking residues such as Gly, Gly-Gly-, Ser, Ser-Ser, or the like, to an immunogenic peptide. The lipidated peptide can then be injected directly in a micellar form, incorporated into a liposome or emulsified in an adjuvant, e.g., incomplete Freund's adjuvant. In one embodiment a particularly effective immunogen comprises palmitic acid attached to alpha and epsilon amino groups of Lys, which is attached via linkage, e.g., Ser-Ser, to the amino terminus of the immunogenic peptide.
[0082] The peptides of the invention can be prepared in a wide variety of ways. Because of their relatively short size, some such peptides (discrete epitopes or polyepitopic peptides) can be synthesized in solution or on a solid support in accordance with conventional techniques. Various automatic synthesizers are commercially available and can be used in accordance with known protocols. See, for example, Stewart and Young, Solid Phase Peptide Synthesis, 2d. ed., Pierce Chemical Co. (1984), which is incorporated herein by reference.
[0083] The peptides of the present invention and pharmaceutical and vaccine compositions thereof are useful for administration to mammals, particularly humans, to therapeutically treat and/or prevent infections. For pharmaceutical compositions, the immunogenic peptides of the invention are often administered to an individual already infected with the infectious agent of interest. Those in the incubation phase or the acute phase of infection can be treated with the immunogenic peptides separately or in conjunction with other treatments, as appropriate. In therapeutic applications, compositions are administered to a patient in an amount sufficient to elicit an effective CTL response to the infectious agent's antigen and to cure or at least partially arrest symptoms and/or complications. An amount adequate to accomplish this is defined as a therapeutically effective dose or unit dose. Amounts effective for this use will depend on, e.g., the peptide composition, the manner of administration, the stage and severity of the disease being treated, the weight and general state of health of the patient, and the judgment of the prescribing physician. Generally for humans the dose range for the initial immunization (that is for therapeutic or prophylactic administration) is from about 1.0 g to about 20,000 g of peptide for a 70 kg patient, typically about 50 g, 100 g, 150 g, 200 g, 250 g, 300 g, 400 g, or 500 g, 1000 g, 2000 g, 5,000 g, 10, 000 g, 15,000 g, or 20,000 g, sometimes followed by boosting dosages in the same or dose range, though not necessarily the same actual dose, pursuant to a boosting regimen over weeks to months depending upon the patient's response and condition by measuring specific CTL activity in the patient's blood.
[0084] The identification of patients for treatment with such vaccine compositions and of population segments for prophylactic administration of such vaccine compositions is well within the skill of one of ordinary skill in the art. For therapeutic use, administration should begin at the first sign of infection or shortly after diagnosis in the case of acute infection. This is followed by boosting doses until at least symptoms are substantially abated and for a period thereafter. In chronic infection, loading doses followed by boosting doses may be required.
[0085] The peptide compositions can also be used for the treatment of chronic infection and to stimulate the immune system to eliminate, e.g., virus-infected cells in carriers. It is often important to provide an amount of immuno-potentiating peptide in a formulation and mode of administration sufficient to effectively stimulate a cytotoxic T-cell response. Thus, for treatment of chronic infection, immunizing doses followed by boosting doses at established intervals, e.g., from one to four weeks, may be required, possibly for a prolonged period of time, to effectively immunize an individual.
[0086] Frequently it is desirable to prepare a cocktail containing at least two, or at least three, or five or more antigens from an infectious agent to ensure that the vaccine is effective for a broad range of recipients. In addition to the primary antigenic activity of a peptide, it is sometimes also useful to determine if non-immunized subjects also exhibit an immune response to the peptide. A cocktail of immunogenic peptides to be used as a vaccine is sometimes selected to include at least 2 or at least 3 proteins that react with serum from immunized subjects and do not react with serum from non-immunized subjects.
[0087] Delivery of the compositions of the invention can be by any methods familiar to those of skill in the art, including oral, inhalation, topical, and injection methods. Frequently, the pharmaceutical compositions are administered parenterally, e.g., intravenously, subcutaneously, intradermally, or intramuscularly. Thus, the invention provides compositions for parenteral administration which comprise a solution of the immunogenic peptides dissolved or suspended in an acceptable carrier, preferably an aqueous carrier. A variety of aqueous carriers may be used, e.g., water, buffered water, 0.8% saline, 0.3% glycine, hyaluronic acid and the like. These compositions may be sterilized by conventional, well known sterilization techniques, or may be sterile filtered. The resulting aqueous solutions may be packaged for use as is, or lyophilized, the lyophilized preparation being combined with a sterile solution prior to administration. The compositions may contain pharmaceutically acceptable auxiliary substances as required to approximate physiological conditions, such as pH adjusting and buffering agents, tonicity adjusting agents, wetting agents and the like, for example, sodium acetate, sodium lactate, sodium chloride, potassium chloride, calcium chloride, sorbitan monolaurate, triethanolamine oleate, etc.
[0088] The compositions of the invention may also be administered via liposomes. Liposomes include emulsions, foams, micelles, insoluble monolayers, liquid crystals, phospholipid dispersions, lamellar layers and the like. In these preparations the peptide to be delivered is incorporated as part of a liposome, alone or in conjunction with a molecule which binds to, e.g., a receptor prevalent among lymphoid cells, such as monoclonal antibodies which bind to the CD45 antigen, or with other therapeutic or immunogenic compositions. Thus, liposomes either filled or decorated with a desired peptide of the invention can be directed to the site of lymphoid cells, where the liposomes then deliver the selected therapeutic/immunogenic peptide compositions. Liposomes for use in the invention are formed from standard vesicle-forming lipids, which generally include neutral and negatively charged phospholipids and a sterol, such as cholesterol. The selection of lipids is generally guided by consideration of, e.g., liposome size, acid lability and stability of the liposomes in the blood stream. A variety of methods are available for preparing liposomes, as described in, e.g., Szoka, et al., Ann. Rev. Biophys. Bioeng. 9:467 (1980), U.S. Pat. Nos. 4,235,871, 4,501,728, 4,837,028, and 5,019,369. Other types of adjuvants and emulsions can also be used such as SAF-1, PROVAX and Tomatine. Also alum can be used to help stimulate the immune response against the formulated protein or peptide antigens.
[0089] For solid compositions, conventional nontoxic solid carriers may be used which include, for example, pharmaceutical grades of mannitol, lactose, starch, magnesium stearate, sodium saccharin, talcum, cellulose, glucose, sucrose, magnesium carbonate, and the like. For oral administration, a pharmaceutically acceptable nontoxic composition is formed by incorporating any of the normally employed excipients, such as those carriers previously listed, and generally 0.01-95% of active ingredient, that is, one or more peptides of the invention, and more preferably at a concentration of 0.1% to 75%, or 0.2%-50% or 1%-20%.
[0090] For aerosol administration, the immunogenic peptides are generally supplied in finely divided form along with a surfactant and propellant. Typical percentages of peptides are 0.01%-20% by weight, or 1%-10%. The surfactant must, of course, be nontoxic, and is generally soluble in the propellant. Representative of such agents are the esters or partial esters of fatty acids containing from 6 to 22 carbon atoms, such as caproic, octanoic, lauric, palmitic, stearic, linoleic, linolenic, olesteric and oleic acids with an aliphatic polyhydric alcohol or its cyclic anhydride. Mixed esters, such as mixed or natural glycerides may be employed. The surfactant may constitute 0.1%-20% by weight of the composition, commonly 0.25-5%. The balance of the composition is ordinarily propellant. A carrier can also be included, as desired, as with, e.g., lecithin for intranasal delivery.
[0091] The peptides of the invention can also be expressed by attenuated viral hosts, such as vaccinia or fowlpox. This approach involves the use of vaccinia virus as a vector to express nucleotide sequences that encode the peptides of the invention. Vaccinia vectors and methods useful in immunization protocols are described in, e.g., U.S. Pat. No. 4,722,848. Another vector is BCG (Bacille Calmette Guerin). BCG vectors are described, e.g., in Stover, et al. (Nature 351:456-460 (1991)), which is incorporated herein by reference. A wide variety of other vectors useful for therapeutic administration or immunization of the peptides of the invention, e.g., Salmonella typhi vectors and the like, will be apparent to those skilled in the art from the description herein.
[0092] For therapeutic or immunization purposes, peptides of the invention can be administered in the form of nucleic acids encoding one or more of the peptides of the invention. The nucleic acids can encode a peptide of the invention and optionally one or more additional molecules. A number of methods are conveniently used to deliver nucleic acids to a patient. For instance, nucleic acid can be delivered directly, as naked DNA. This approach is described, for instance, in Wolff, et al., Science 247: 1465-1468 (1990) as well as U.S. Patent Nos. 5,580,859 and 5,589,466, each of which is incorporated herein by reference. Nucleic acids can also be administered using ballistic delivery as described, for instance, in U.S. Pat. No. 5,204,253. Particles comprised solely of DNA can be administered. Alternatively, DNA can be adhered to particles, such as gold particles. As with delivery of peptides, it is frequently desirable to prepare a cocktail containing at least two, or at least three, or five or more nucleic acids encoding antigenic peptides from an infectious species to ensure that the DNA vaccine is effective for a broad range of recipients.
[0093] The nucleic acids can also be delivered complexed to cationic compounds, such as cationic lipids. Lipid-mediated gene delivery methods are described, for instance, in WO96/18372; WO 93/24640; Mannino & Gould-Fogerite, BioTechniques 6(7): 682-691 (1988); Rose U.S. Pat No. 5,279,833; WO 91/06309; and Feigner, et al., Proc. Natl. Acad. Sci. USA 84: 7413-7414 (1987), each of which is incorporated herein by reference.
[0094] Purified-plasmid DNA can be prepared for injection using a variety of formulations. The simplest of these is reconstitution of lyophilized DNA in sterile phosphate-buffer saline (PBS). A variety of methods have been described, and new techniques may become available. As noted above, nucleic acids are conveniently formulated with cationic lipids. In addition, glycolipids, fusogenic liposomes, peptides and compounds referred to collectively as protective, interactive, non-condensing (PINC) could also be complexed to purified plasmid DNA to influence variables such as stability, intramuscular dispersion, or trafficking to specific organs or cell types.
[0095] The immunologic compositions will contain effective amounts of one or more of the identified antigens along with suitable excipients. Vaccines for injection will typically contain excipients and additional ingredients to confer stability. The nature of the composition will depend on the route of administration which may be, for example, intravenous, intramuscular, subcutaneous, or intraperitoneal injection, or may be transmucosal, transdermal, or oral. The design of compositions for vaccines is well established, and is described, for example, in Remington's Pharmaceutical Sciences, latest edition, Mack Publishing Co., Easton, Pa., and in Plotkin and Orenstein's book entitled Vaccines, 4th Ed., Saunders, Philadelphia, PA (2004), each of which is incorporated herein by reference.
[0096] Immunizations with individual proteins, as opposed to inactivated viral particles, may require adjuvants in order to elicit a strong immune response. While mineral oil may suffice, the use of squalane emulsions stabilized by linear amphipathic polymers called pluronic polyols has been reported to be superior for eliciting an immune response. See Hunter, et al., Vaccine, 20 Suppl. 3, S7-12 (2002), which is incorporated herein in its entirety by reference. Furthermore, liposome formulations may be advantageously used to increase immunological response to proteins. See Lidgate, et al., Pharm. Research, 5, pg. 759-764 (1988); Hjorth, et al, Vaccine 15, 541-46 (1997), each of which is incorporated herein in its entirety by reference. General methods and protocols for administration of vaccines are also described in Plotkin and Orenstein, Vaccines, 4th ed.
[0097] The antigens provided by the invention are also useful for diagnostic purposes as well as for administration to induce immunity. A specific reaction to one or more, or two or more, or preferably three or more specific antigens identified by the above methods can be used to detect or quantify antibodies to the infectious agent, which allows rapid identification of the agent and the specific strain of the agent in an infected subject. An array of antigens can be used to very precisely distinguish a particular strain of an infectious agent. This permits detection of an infectious agent in an exposed subject even before symptoms have appeared. It permits determination of whether a subject has immunity to a specific infectious agent, so unnecessary immunization can be avoided. It also enables the identification of antibiotic-resistant bacterial infections or antiviral-resistant viral infections, for example, thus permitting a physician to avoid administering an ineffective drug and to quickly select an appropriate drug or therapy. Furthermore, it permits the user to identify specific disease states: the serum profile in a patient with chronic tuberculosis will be different from that in a patient with a new or active infection, and the disease state can thus be more precisely characterized using the antigens provided by the invention diagnostically.
[0098] The present invention also encompasses antibodies to proteins of the present invention and arrays of such antibodies. Antibodies may be made by any suitable means, for example, in laboratory animals such as rabbits, mice or domestic dogs. An antigen comprising a protein of the present invention may be mixed with incomplete Freund's adjuvant, alum adjuvant or with no adjuvant (PBS only) and injected into the laboratory animal, using one or more injections. Any form of the antigen can be used to generate the antibody that is sufficient to generate a specific antibody for a given antigen. The eliciting antigen may be a single epitope, multiple epitopes, or the entire protein alone or in combination with one or more immunogenicity enhancing agents known in the art. The eliciting antigen may be an isolated full-length protein, a cell surface protein (e.g., immunizing with cells transfected with at least a portion of the antigen), or a soluble protein (e.g., immunizing with only the extracellular domain portion of the protein).
[0099] As used herein, antibodies refers to both intact immunoglobulins and to immunologically reactive fragments of such antibodies, such as Fab, Fab, F(ab2), fragments, single-chain variable regions produced recombinantlyi.e., sFv forms, and any other fragments which are able specifically to recognize epitopes.
[0100] In some embodiments, a monoclonal antibody is preferred. Methods to generate monoclonal antibodies are well known in the art, and are generally described in Janeway, et al., Immunobiology, 5th ed., Garland Publishing, New York, N.Y. (2001), which is incorporated herein by reference. Methods to immobilize antibodies to produce arrays are also known in the art, such as application to a retentive surface such as nitrocellulose.
[0101] The antibodies can be screened for binding to normal or phenotypic variant forms of an antigenic protein. See e.g., ANTIBODY ENGINEERING: A PRACTICAL APPROACH (Oxford University Press, 1996), which is incorporated herein by reference. These monoclonal antibodies will usually bind with at least a Ka of about 1 M, more usually at least about 300 nM, typically at least about 30 nM, often at least about 10 nM, frequently at least about 3 nM or better, usually determined by ELISA. Included in the definition of monoclonal antibodies are those that are chimeric forms (i.e., comprise portions of the heavy and light chains from different species) or are humanized or otherwise adapted to a particular subject by standard humanization or subject adaptation techniques.
[0102] The antibodies provided herein are useful in diagnostic applications, as well as in conferring passive immunity. They include isolated antibodies produced and at least partially purified using methods well known in the art. These antibodies can be used to detect or quantify the infectious agent from which the antigen was obtained; for example, they can be used to detect a bioweapon infectious agent in a subject or in a potentially contaminated material, because they can be very rapidly generated for a new strain. They may also be used to distinguish between strains of the infectious agent for therapeutic or epidemiology purposes, or to identify specific strains such as those that are sensitive to or insensitive to specific drugs. Arrays of the antibodies are useful for identifying a specific strain of an infectious agent. The antibodies are also useful reagents for antigen purification.
[0103] The following examples are offered to illustrate but not to limit the invention. In these examples, the vaccinia strain used was the WR strain. Sequences of the open reading frames of the genome of this strain are deposited at GenBank with the designations VACWR followed by a number. A list of the loci of the open reading frames is found in Table 8, which follows these examples. The orthologs of the open reading frames listed in Table 8 for the WR strain that are present in the Copenhagen strain are also characterized by their sequences in GenBank where they have the designations shown in the second column of Table 8.
[0104] It will be seen that one of the loci in the WR strain, VACWR148, does not have a corresponding ortholog in the Copenhagen strain; it corresponds in part to the antigen having the designation A29L in Variola major and was initially identified as such. On closer scrutiny, WR148 shows a strong immuno-dominant antigenic response but does not map to a single gene in related species. Rather, the WR146, WR147, WR148, and WR149 genes correspond to an A-type inclusion protein group or ATI locus proteins. The ATI locus proteins correspond to A26L and A27L in cowpox, and to A26L, A27L, A28L, A29L and A30L in variola.
[0105] In the examples and in the claims, the nomenclature corresponding to the Copenhagen ortholog is used for the other genes and gene products, and ATI locus genes or ATI locus proteins for the VACWR148 antigens. The correspondence to the WR strain used in the example can be found in Table 8.
EXAMPLE 1
Preparation of Vector and Inserts
[0106] A linear T7 vector encoding an N-terminal histidine tag and a C-terminal HA tag was generated by extensive restriction digestion followed by PCR; this procedure reduced the amount of residual circular vector and background colonies to nearly zero when it is transformed without complementary insert into chemically competent E. coli.
[0107] The plasmid used to generate the linear recombination vector pXT7, is shown in
[0108] In more detail, plasmid pXT7 (10 g; 3.2 kb, KanR) was linearized with BamH1 (0.1 g/l DNA, 0.1 mg/ml BSA, 0.2 U/l BamH1, 37 C., 4 h; additional BamH1 was added to 0.4 U/l, 37 C., overnight). The digest was purified (Qiagen PCR purification kit), quantified by fluorometry and verified by agarose gel electrophoresis (1 g). One nanogram of this material was used to generate the linear acceptor vector in a 50 l-PCR (Primers, 0.5 M each: 5CTACCCATACGATGTTCCGGATTAC, 5CTCGAGCATATGCTTGTCGTCGTCG; 0.02 U/l Taq DNA polymerase [Fisher Scientific, buffer A]; 0.1 mg/ml gelatin [Porcine, Bloom 300; Sigma, G-1890]; 0.2 mM each dNTP; initial denaturation: 95 C., 5 min; 30 cycles: 95 C., 0.5 min/50 C., 0.5 min/72 C., 3.5 min; final extension: 72 C., 10 min). The PCR product was visualized by agarose gel electrophoresis (3 l), purified (Qiagen PCR purification kit), and quantified by fluorometry using picogreen (Molecular Probes) according to the manufacturer's instructions. Each batch of linear acceptor vector was checked for background KanR transformants (no KanR transformant per 40 ng).
[0109] ORF's from vaccinia virus and F. tularensis were amplified using gene specific primers containing 33 nucleotide extensions complementary to the ends of the linear T7 vector.
[0110] One to ten nanograms genomic DNA were used as template in a 50 l-PCR: Primers, 0.5 M each (5CATATCGACGACGACGACAAGCATATGCTCGAG [20-mer ORF specific at 5-end]; 5ATCTTAAGCGTAATCCGGAACATCGTATGGGTA [20-mer ORF specific at 3-end]); 0.02 U/l Taq DNA polymerase [Fisher Scientific, buffer A]; 0.1 mg/ml gelatin [Porcine, Bloom 300; Sigma, G-1890]; 0.2 mM each dNTP; initial denaturation: 95 C., 5 min; 30 cycles: 20 sec at 95 C., 0.5 min at 50 C., 1 min per 1 kb at 72 C., 1 to 3 min on average based on ORF size; final extension: 72 C. for 10 min). Those PCR products more difficult to produce were re-amplified using 0.5 min annealing at 45 and 40 C. instead of 50 C. The PCR products were purified (Qiagen PCR purification kit), quantified by fluorometry using picogreen (Molecular Probes, Eugene Oreg.) and visualized to validate size and purity by agarose gel electrophoresis.
[0111] Each open reading frame was amplified from genomic template using gene specific primers. The 5 oligonucleotide contained 53 nucleotides; of these 33 nucleotides comprise the 5 universal end sequence and the other 20 nucleotides make up the gene-specific sequence. The first start codon, ATG, is upstream of the polyhistidine tag on the linear vector, and each open reading frame also begins with ATG. The 3-custom oligonucleotide also contains 53 nucleotides; of these, 33 comprise the 3 universal end sequence and the other 20 nucleotides are specific to the gene-of-interest. A stop codon sequence, TTA, was added to the end of the gene sequence to achieve translational termination of the expressed gene.
[0112] The primers are shown in
EXAMPLE 1A
[0113] Applying these methods to the vaccinia virus required preparation of primers for 213 genes, from which 211 PCR products were isolated (>99%). All 211 of these were cloned, and 181 of the products were submitted for sequencing; 93% (169 out of 181) provided the predicted sequence.
[0114] EXAMPLE 1B
[0115] Similarly, applying the methods to P. falciparum required preparation of primers for 720 genes. From these, 462 PCR products were obtained (64%), and 266 clones were produced (58%). A set of these (63) were submitted for sequencing, with 97% giving the expected sequence.
[0116] EXAMPLE 1C
[0117] The above methods were applied to Mycobacterium tuberculosis for which primers for 108 genes were prepared. From these, 87 PCR products were obtained (80%) and 80 clones were produced (92%), each of which had an anti-His tag on one end and an anti-HA tag on the other. Sequencing confirmed that 70 out of 79 tested (88%) contained the expected sequence. In most of the proteins produced, both the His and HA tags were accessible for binding, but in a number of cases, only one tag was bound; generally, where only one was accessible, it was the His tag that remained accessible for binding, and the HA epitope tag that was inaccessible.
[0118] This method was expanded to express 312 genes from Mycobacterium tuberculosis H37Rv, out of a genome of about 4,000 genes.
EXAMPLE 1D
[0119] The above methods were applied to F. tularensis for which primers for 1933 genes were prepared. From these, 1842 PCR products were obtained (95%) and 1720 clones were produced (93%). Sequencing of 684 of these showed that 643 (94%) contained the expected sequence.
EXAMPLE 2
In Vivo Recombination and Colony Selection
[0120] Mixtures of PCR amplified ORF's and linear T7 vector of Example 1 were mixed and introduced into chemically competent E. coli, resulting in transformed colonies containing plasmid with insert. This high efficiency recombination cloning method resulted in in-frame directional insertion of ORF.
[0121] The competent cells were prepared in our laboratory by growing DH5a cells at 18 C. in 500 ml SOB medium (2% tryptone, 0.5% yeast extract, 10 mM NaCl, 2.5 mM KCl, and 20 mM MgSO4) to an optical density of 0.5-0.7 O.D. The cells were washed and suspended in 10 ml pre-chilled PCKMS buffer (10 mM PIPES, 15 mM CaCl.sub.2, 250 mM KCl, 55 mM MnCl.sub.2, and 5% sucrose, pH 6.7) on ice and 735 l DMSO was added dropwise with constant swirling. The competent cells were frozen on dry ice ethanol in 100 l aliquots and stored at 80 C.
[0122] Each transformation consisted of: 10 l competent DH5 (prepared as above in our laboratory with efficiency of 10.sup.9 cfu/mg of supercoiled plasmid DNA) and 10 l DNA mixture (40 ng PCR-generated linear vector, 10 ng PCR-generated ORF fragment; molar ratio 1:1, vector: 1 kb ORF fragment). The mixture was incubated on ice, 45 min; heat shocked (42 C., 1 min); chilled on ice, 1 min; mixed with 250 l SOC medium (2% tryptone, 0.55% yeast extract, 10 mM NaCl, 10 mM KCl, 10 mM MgCl.sub.2, 10 mM MgSO.sub.4, 20 mM glucose); incubated 37 C., 1 h; diluted into 3 ml LB (Luria Bertani Medium) supplemented with 50 g kanamycin/ml (LB Kan 50), and incubated with shaking overnight. Single colonies were obtained from the overnight culture by streaking on LB Kan 50 agar. From each transformation, 2-3 colonies were selected for further analysis. Plasmid DNA obtained from Qiagen miniprep was visualized by gel electrophoresis for selection of clones with insert.
[0123] Transformation of the DH5a competent cells was accomplished with a mixture of PCR fragments and linear vector in a molar ratio of 1:1 and with 50 ng of total DNA used in the transformation. The competent cells were transformed, grown overnight and observed for turbidity due to bacterial growth before plating and colony selection. Under these conditions cloning efficiency was >90%, but if the cells were plated on the day of transformation the observed success rate was lower. The rate of successful transformation progressively declined as the total DNA used for transformation was reduced to 25 and 10 ng (not shown).
[0124]
[0125] The overnight cultures shown in
EXAMPLE 3
In Vitro Transcription and Translation Detection of Protein
[0126] The proteins encoded on the plasmids shown in
[0127] For the results shown in
[0128] Non-denatured proteins from the cell-free reactions could also be detected on dot-blots. (
EXAMPLE 4
Microarrays and Serological Screening
[0129] Commercially available Vaccinia Immune Globulin (VIG) from Cangene Corp (Winnipeg, Canada) was used. VIG is the immunoglobulin fraction of hyperimmune sera pooled from multiple donors. It is used as an emergency therapy for people undergoing systemic viraemia and other adverse reactions to vaccinia vaccination.
[0130] For immuno-dot-blots, 0.3 Ill volumes of whole RTS reactions were spotted manually onto nitrocellulose membranes and allowed to air dry prior to blocking in 5% non-fat milk powder in TBS-Tween. Blots were probed with VIG, diluted to 1/1,000 in blocking buffer with or without 10% E. coli lysate. Three different batches of VIG were used: lot #1730204 (56 mg/ml), lot #1730208 (53 mg/ml) and lot #1730302 (56 mg/ml). Bound human antibodies were detected by incubation in alkaline phosphatase-conjugated goat anti-human IgA+IgG+IgM (H+L) secondary antibody (Jackson ImmunoResearch) and visualized with nitro-BT developer. Routinely, dot-blots were also stained with both monoclonal anti-polyhistidine (clone His-1; Sigma H-1029) and with monoclonal rat anti-hemagglutinin (clone 3F10; Roche 1 867 423), followed by AP-conjugated goat anti-mouse IgG (H+L) (BioRad) or goat anti-rat IgG (H+L) secondary antibodies (Jackson ImmunoResearch), respectively, to confirm the presence of recombinant protein.
[0131] In vitro transcription/translation reactions set up in a 25 l scale, and control reactions using non-recombinant expression plasmid as the template are also set up to control for the presence of E. coli antigens are used. Immediately after the end of the 5 h synthesis reaction, the proteins were either spotted or arrayed onto nitrocellulose substrates without further purification, or held at 4 C. for no more than 12 h prior to printing. Spotting of RTS reactions was under non-denaturing conditions, and without further purification (
EXAMPLE 5
Microarrays
[0132]
[0133] In vitro transcription/translation reactions were printed, without purification, onto nitrocellulose-coated glass slides and probed with VIG with and without 10% E. coli lysate. The control spots consist of RTS reactions with non-recombinant expression plasmid as the vector. An arbitrary cut-off, over which staining can be considered positive, was established by calculating the mean and standard deviation of the fluorescence intensity of the control spots. As can be seen when lysate is present in the VIG, the same proteins that were detected in the immuno-dot-blot are also detected by microarray. The fluorescently conjugated secondary antibodies provide a wider range of signal intensities than seen with the immuno-dot-blots. Moreover the microarrays also appear to give greater sensitivity than the immuno-dot-blots, since we have observed several cases where proteins that were detected in arrays were below the threshold of detection in the dot-blots (not shown).
[0134]
EXAMPLE 6
Preparation of Plasmids from Transformation Mixtures
[0135] Rather than selecting individual colonies for further assessment as in Examples 2-5, the transformation mixture, obtained as described in Example 2 was used as the source of plasmids containing the desired inserts. As above, each transformation consisted of: 10 l competent DH5 and 10 l DNA mixture (40 ng PCR-generated linear vector, 10 ng PCR-generated ORF fragment from vaccinia; molar ratio 1:1, vector: 1 kb ORF fragment). The mixture was incubated on ice, 45 min; heat shocked (42 C., 1 min); chilled on ice, 1 min; mixed with 250 l SOC medium (2% tryptone, 0.55% yeast extract, 10 mM NaCl, 10 mM KCl, 10 mM MgCl.sub.2, 10 mM MgSO.sub.4, 20 mM glucose); incubated 37 C., 1 h; diluted into 3 ml LB (Luria Bertani Medium) supplemented with 50 g kanamycin/ml (LB Kan 50), and incubated with shaking overnight. The plasmid was isolated and purified from this culture, without colony selection. The resulting plasmid templates were translated substantially as described in the foregoing examples and transferred to immuno-dot-blots as follows:
[0136] Plasmid templates used for in vitro transcription/translation were prepared using the Qiagen miniprep kits, including the optional step which contains protein denaturants to deplete RNase activity. If this step is not included, the level of expression in the in vitro transcription/translation reaction was low and inconsistent.
[0137] In vitro transcription/translation reactions (RTS 100 E. coli HY kits from Roche) with 25 l reaction volumes were set up in 0.2 ml PCR 12-well strip tubes and incubated for 5 h at 30 C. according to the manufacturer's instructions. The proteins encoded on the T7 plasmids representing a set of 8 vaccinia and 40 F. tularensis proteins were expressed in an E. coli based cell-free in vitro transcription/translation system that was supplemented with T7 RNA polymerase. The 25 l in vitro transcription/translation reactions were incubated for 4 hours at 37 C., the crude unpurified reactions were resolved on SDS polyacrylamide gels, and the gels were blotted and probed with anti-polyhistidine antibody (
[0138] For immuno-dot-blots, 0.3 l volumes of whole RTS reactions were spotted manually onto nitrocellulose membranes and allowed to air dry prior to blocking in 5% non-fat milk powder in TBS containing 0.05% Tween 20. Blots were probed with vaccinia immune globulin (VIG) from Cangene Corporation (Winnipeg, Manitoba, Canada) diluted to 1/1000 in blocking buffer with or without 10% E. coli lysate. Three different batches of VIG were used: lot #1730204 (56 mg/ml), lot #1730208 (53 mg/ml) and lot #1730302 (56 mg/ml). Bound human antibodies were detected by incubation in alkaline phosphatase-conjugated goat anti-human IgA+IgG+IgM (H+L) secondary antibody (Jackson ImmunoResearch) and visualized with nitro-BT developer. Routinely, dot-blots were also stained with both monoclonal anti-polyhistidine (clone His-1; Sigma H-1029) and with monoclonal rat anti-hemagglutinin (clone 3F10; Roche 1 867 423), followed by AP-conjugated goat anti-mouse IgG (H+L) (BioRad) or goat anti-rat IgG (H+L) secondary antibodies (Jackson ImmunoResearch), respectively, to confirm the presence of recombinant protein. For microarrays 10 l of 0.125% Tween 20 was mixed with 15 l RTS reaction (to give a final concentration of 0.05% Tween), and 15 l volumes were transferred to 384-well plates. The plates were centrifuged 1600g to pellet any precipitate, and supernatant printed without further purification onto nitrocellulose-coated FAST glass slides (Schleicher & Schuell Bioscience) using an Omni Grid 100 microarray printer (Gene Machines). For all staining, slides were first blocked for 30 mins in protein array blocking buffer (Schleicher & Schuell) and stained with the same primary and secondary antibodies as for the dot-blots (with Cy3 conjugated secondary antibodies from Jackson) and scanned in a laser confocal scanner. Fluorescence intensities were quantified using QuantArray software (GSI Lumonics, Inc). VIG has high titers of anti-E. coli antibodies that mask any antigen-specific responses when using whole RTS reactions on dot-blots and arrays. This was overcome by the adsorption of VIG against immunoblots of E. coli lysates, or by the addition of E. coli lysate to the VIG. In the former method, E. coli was solubilized in SDS PAGE sample buffer and the lysate resolved on preparative gels prior to transfer to Optitran nitrocellulose membranes (Schleicher & Schuell). The blots were then cut into small (55 mm) pieces and blocked in 5% non-fat milk powder for 1 h. The pieces were then rinsed and placed into VIG previously diluted to 1/1000 in blocking buffer, and incubated for 1 h with constant agitation. E. coli lysate was produced from a lliter stationary phase culture of E. coli (DH5) resuspended in 25 ml TBS-Tween and sonicated with a 2 cm diameter probe. One ml aliquots were stored at 80 C. Mouse sera, which lack endogenous anti-E. coli reactivity, do not require pre-treatment with E. coli lysate to reduce background.
[0139] Non-denatured proteins from the cell-free reactions could also be detected on immuno-dot-blots (
[0140] It is apparent from the blot in panel12C that VIG has high titers of anti-E. coli antibody, masking any reactivity to vaccinia proteins. However, the addition of E. coli lysate to VIG (panel 12D) reduces this background to a level such that the detection of the vaccinia protein is possible. Positive proteins on this blot were, A10L, A27L, D8L, D13L, F13L, H3L & HSR, highlighted in red in the caption.
[0141] E. coli lysate treatment of serum was also effective to reduce E. coli background reactivity on microarrays. A pilot microarray consisting of 23 vaccinia and 22 F. tularensis proteins probed with VIG, with and without E. coli lysate is shown in
[0142]
[0143] The antigens in Table 1 are all proteins from the Western Reserve (WR) strain, but are identified herein by the name of their nearest ortholog in the Copenhagen strain of vaccinia virus, since the protein functions are better characterized in that strain. Nevertheless, sequences for each of the ORFs and for the encoded proteins from the WR strain are available in the GenBank database, which is available online at the web address www.ncbi.nlm.nih.gov/gquery/gquery.fcgi. The descriptions set forth in Table 1 match those in the database. The protein and gene sequences for the WR strain are in the Vaccinia WR genome, and can be located in GenBank using the Gene names from Table 1. Proteins that are substantially similar to these and their corresponding gene sequences can be readily identified using the blast utilities available through GenBank.
TABLE-US-00001 TABLE 1 Immuno Reactive Proteins Identified by this Serological Screen TM Domain/Sig. Gene Name Antigen PI Mol. Wt. Description Peptide Reactive in Immunized Mice, Humans & Macaques VACWR129 A10L 6.33 102,283 major core protein No/No VACWR130 A11R 4.81 36,134 hypothetical protein Yes/No VACWR132 A13L 9.96 7,696 structural protein Yes/Yes VACWR156 A33R 5.3 20,506 EEV glycoprotein Yes/Yes VACWR181 A56R 4.05 34,778 hemagglutinin Yes/Yes VACWR187 B5R 4.54 35,108 plaque-size/host range protein Yes/Yes VACWR113 D8L 9.55 35,326 cell surface-binding protein Yes/No VACWR118 D13L 5.10 61,890 rifampicin resistance protein No/No VACWR052 F13L 6.98 41,823 major envelope protein No/No VACWR101 H3L 6.43 37,458 IMV membrane protein Yes/No VACWR103 H5R 7.55 22,270 late transcription factor No/No Reactive in Immunized Humans & Macaques VACWR146/149* A26L 9.40 37,319 A-type inclusion protein No/No Reactive in Immunized Humans & Mice VACWR150 A27L 5.14 12,616 cell fusion protein No/No VACWR059 E3L 5.04 21,504 IFN resistance protein No/No VACWR091 L4R 6.13 28,460 DNA-binding core protein No/No Reactive in Immunized Mice & Macaques VACWR105 H7R 7.27 16,912 hypothetical protein No/No Reactive in Immunized Macaques Only VACWR137 A17L 4.28 22,999 IMV membrane protein Yes/Yes Reactive in Mice Only VACWR122 A3L 6.75 72,624 major core protein No/No VACWR123 A4L 4.68 30,846 Memb. Associated core No/No protein VACWR116 D11L 9.13 72,366 DNA helicase No/No VACWR104 H6R 10.30 36,665 topisomerase No/No VACWR033 K2L 9.73 42,299 serine protease inhibitor No/Yes VACWR028 N1L 4.41 13,961 Hypothetical proteins No/No Reactive in Nave (Non-immunized) Humans VACWR166 A4IL 4.90 25,092 Secreted glycoprotein No/Yes VACWR173 A47L 10.29 28,334 hypothetical protein No/No VACWR184 B2R 6.84 24,628 hypothetical protein No/No VACWR115 D10R 8.12 28,934 NTP phosphoydrolase No/Yes VACWR057 E1L 8.71 55,580 poly(A) polymerase (VP55) No/No VACWR041 F2L 8.64 16,264 dUTP pyrophosphatase No/No VACWR048 F9L 6.72 23,792 Thiroedoxin substrate Yes/Yes VACWR082 G5R 4.93 49,872 Core/assembly protein No/No VACWR085 G7L 7.72 41,920 Structural/core protein No/No VACWR105 H7R 7.27 16,912 hypothetical protein No/No VACWR070 I1L 9.05 35,841 Telomere binding protein No/No VACWR092 L5R 10.32 15,044 Myristylated protein Yes/No VACWR069 O2L 5.27 12,355 glutaredoxin No/No Reactive in Immunized Mice, Humans & Macaques VACWR129 A10L 6.33 102,283 major core protein No/No VACWR130 A11R 4.81 36,134 hypothetical protein Yes/No VACWR132 A13L 9.96 7,696 structural protein Yes/Yes VACWR156 A33R 5.3 20,506 EEV glycoprotein Yes/Yes VACWR181 A56R 4.05 34,778 hemagglutinin Yes/Yes VACWR113 D8L 9.55 35,326 cell surface-binding protein Yes/No VACWR118 D13L 5.10 61,890 rifampicin resistance protein No/No VACWR052 F13L 6.98 41,823 major envelope protein No/No VACWR101 H3L 6.43 37,458 IMV membrane protein Yes/No VACWR103 H5R 7.55 22,270 late transcription factor No/No Reactive in Immunized Humans & Macaques VACWR146/149* A26L 9.40 37,319 A-type inclusion protein No/No Reactive in Immunized Humans & Mice VACWR150 A27L 5.14 12,616 cell fusion protein No/No VACWR091 L4R 6.13 28,460 DNA-binding core protein No/No Reactive in Immunized Mice & Macaques VACWR187 B5R 4.54 35,108 plaque-size/host range protein Yes/Yes VACWR105 H7R 7.27 16,912 hypothetical protein No/No Reactive in Immunized Macaques Only VACWR137 A17L 4.28 22,999 IMV membrane proteins Yes/Yes Reactive in Immunized Mice Only VACWR122 A3L 6.75 72,624 major core protein No/No VACWR123 A4L 4.68 30,846 Memb, associated core protein No/No VACWR116 D11L 9.13 72,366 DNA helicase No/No VACWR059 E3L 5.04 21,504 Adenosine deaminase No/No VACWR104 H6R 10.30 36,665 topisomerase No/No VACWR033 K2L 9.73 42,299 serine protese inhibitor No/Yes VACWR028 N1L 4.41 13,961 Hypothetical prtoeins No/No
[0144] The proteins eliciting very strong seropositive reactions with VIG include A14L, A27L, H5R, D8R, D13L, DBL, H3L and F13L. Those proteins having moderate immunoreactivity were identified as A10L, A11R, L1R, B5R, A17L, 115L, F5L, A34L, A36R, A56R, and A13L. An additional protein giving a very strong seropositive response with VIG has also been identified; it is referred to as VACWR148, and has no close ortholog in the Copenhagen strain but is homologous to a protein named A29L in variola major. This protein has not previously been identified as antigenic and is referred to as an ATI locus protein herein.
[0145] By way of example only and without limiting the scope of proteins or DNA sequences encompassed by the invention, some of the closest orthologs for some of the immunoactive proteins identified by the present method include:
[0146] VACWR101 (VACV-COP H3L) Additional Orthologs: [0147] VACV-MVA:MVA093L [0148] RPXV-UTR:RPXV-UTR_090 [0149] VACV-AMVA:AMVA095 [0150] CPXV-GRI:J3L [0151] VACV-TAN:Tan-TH3L [0152] VARV-GAR: J3L [0153] VARV-BSH:I3L [0154] VARV-IND:I3L CMLV [0155] CMS:98L
[0156] VACWR118 (VACV-COP D13L) Additional Orthologs: VACV [0157] MVA:MVA110L [0158] VACV-TAN: an-TD15L VACV [0159] AMVA:AMVA112 [0160] CPXV-GRI:E13L [0161] RPXV-UTR:RPXV-UTR 107 [0162] VARV-BSH:N3L [0163] VARV-IND: N3 L [0164] CMLV-CMS:115L CMLV [0165] M96: CMLV116
[0166] VACWR 113 (VACV-COP D8L) Additional Orthologs: RPXV [0167] UTR:RPXV-UTR_102 [0168] VACV-MVA:MVA105L [0169] VACV-AMVA: AMVA107 [0170] VACV-TAN:Tan-TD8L [0171] VARV-IND:F8L [0172] VARV-BSH:F8L [0173] VARV-GAR:F8L [0174] ECTV-NAV:EV-N-114 [0175] ECTV-MOS:EVM097
[0176] VACWR052 (VACV-COP F13L) Additional Orthologs: VACV [0177] TAN: an-TF13L [0178] ECTV-NAV:EV-N-53 [0179] ECTV-MOS:EVM036 [0180] CPXV-GRI: G13L [0181] RPXV-UTR:RPXV-UTR 041 [0182] VACV-AMVA:AMVA045 [0183] VACV-MVA:MVA043L [0184] CPXV-BR:V061 [0185] VARV-GAR:E13L
[0186] VACWR103 (VACV-COP H5R) Additional Orthologs: RPXV [0187] UTR:RPXV-UTR_092 [0188] VACV-TAN:Tan-TH6R [0189] VACV-AMVA:AMVA097 [0190] VACV-MVA:MVA095R [0191] CPXV-GRI: J5R [0192] MPXV-ZRE:H5R [0193] VARV-BSH:I5R [0194] CPXV-BR:V114 [0195] VARV-GAR: J5R
[0196] VACWR187 (VACV-COP B5R) Additional Orthologs: RPXV [0197] UTR:RPXV-UTR 167 [0198] VACV-TAN:Tan-TB5R [0199] VACV-MVA:MVA173R [0200] VACV-AMVA:AMVA173 [0201] CPXV-GRI:B4R [0202] MPXV-ZRE:B6R [0203] ECTV-MOS:EVM155 [0204] ECTV-NAV:EV-N-182 [0205] VARV-GAR:H7R
[0206] VACWR149 +VACWR146 (VACV-COP A26L) Additional Orthologs: RPXV [0207] UTR:RPXV-UTR 134 [0208] VACV-MVA:MVA137L [0209] VACV-AMVA:AMVA139 [0210] CPXV-GRI: A27L [0211] VACV-TAN:an-TA35L [0212] MPXV-ZRE: A28L [0213] CMLV-M96:CMLV145 [0214] CMLV-CMS:143L [0215] CPXV-BR: V161
[0216] VACWR129 (VACV-COP A10L) Additional Orthologs: VACV [0217] MVA:MVA121L [0218] VACV-AMVA:AMVA123 [0219] RPXV-UTR:RPXV-UTR 118 [0220] CPXV-GRI:A11L [0221] VACV-TAN:an-TA11L [0222] CMLV-M96:CMLV127 [0223] CMLV-CMS:126L [0224] VARV-GAR:A11L [0225] VARV-BSH: A11L
[0226] VACWR130 (VACV-COP Al 1R) Additional Orthologs: VACV [0227] AMVA:AMVA124 [0228] VACV-MVA:MVA122R CPXV [0229] BR:V143 [0230] CPXV-GRI: A12R [0231] MPXV-ZRE: A12R [0232] RPXV-UTR:RPXV-UTR 119 [0233] VACV-TAN:an-TA12R [0234] ECTV-NAV:EV-N-131 [0235] ECTV-MOS:EVM114
[0236] VACWR181 (VACV-COP A56R) Additional Orthologs: VACV [0237] AMVA:AMVA167 [0238] VACV-MVA:MVA165R [0239] VACV-TAN:an-TA66R [0240] CPXV-GRI: A5 8R [0241] MPXV-ZRE:B2R [0242] CMLV-CMS: 173R [0243] VARV-GAR:K9R [0244] CMLV-M96: CMLV176 [0245] VARV-BSH:J7R
[0246] VACWR091 (VACV-COP L4R) Additional Orthologs: [0247] VACV-MVA:MVA083R [0248] RPXV-UTR:RPXV-UTR_080 [0249] VACV-AMVA: AMVA085 [0250] CPXV-BR:V102 [0251] CPXV-GRI:N4R [0252] VACV-TAN:Tan-TL4R [0253] VARV-IND:M4R [0254] CMLV-M96:CMLV089 [0255] VARV-BSH:M4R [0256] CMLV-CMS: 88R
[0257] VACWR156 (VACV-COP A33R) Additional Orthologs: [0258] RPXV-UTR:RPXV-UTR_141 [0259] CPXV-GRI: A34R [0260] VACV-TAN:R(TA43R) [0261] VACV-MVA:MVA144R [0262] VACV-AMVA:AMVA146 [0263] CMLV-M96:CMLV152 [0264] CMLV-CMS:150R [0265] CPXV-BR:V168 [0266] MPXV-ZRE:A35R
[0267] Abbreviations used to describe these orthologs: [0268] VACV-Cop=vaccinia virus strain Copenhagen [0269] VACV MVA=vaccinia virus strain modified virus ankra [0270] VACV-AMVA=Vaccinia virus strain Acambis 3000 MVA [0271] VACVWR=vaccinia virus strain Western Reserve [0272] VACV-TAN=Vaccinia virus strain Tian Tan [0273] CPXV-GRI=cowpox strain GRI-90 [0274] RPV-UTR=Rabbitpox virus strain Utrecht [0275] VARV-GAR=variola minor virus strain Garcia [0276] VARV-BSH=variola major virus strain Bangladesh [0277] VARV-IND=variola major virus strain India [0278] CMLV-CMS=Camelpox virus strain CMS [0279] CMLV-M96=Camelpox virus strain M96 [0280] ECTV-NAV=Ectromelia virus strain Naval (unpublished) [0281] ECTV-MOS=Ectromelia virus Moscow strain [0282] CPXV-BR=Cowpox virus strain Brighton Red [0283] MPXV-ZRE=Monkeypox virus strain Zaire-96-1-16
[0284] Based on the foregoing, a suitable immunologic composition would comprise at least three proteins selected from the group of vaccinia proteins identified herein as antigenic, which group includes ATI locus proteins, A10L, A11R, A13L, A33R, A56R, B5R, D8L, D13L, F13L, H3L, H5R, A26L, A27L, E3L, L4R, H7R, A17L, A3L, A4L, D11L, H6R, K2L, N1L, A41L, A47L, B2R, D10R, E1L, F2L, F9L, GSR, G7L, H7R, I1L, L5R, and O2L. A second immunologic composition for the present invention comprises at least three proteins selected from those active in at least one immunized mammalian species tested, which proteins include ATI locus proteins, A10L, A11R, A13L, A33R, A56R, B5R, D8L, D13L, F13L, H3L, H5R, A26L, A27L, E3L, L4R, H7R, A17L, A3L, A4L, D11L, H6R, K2L, and N1L. A third immunologic composition within the present invention comprises at least three proteins selected from the group which are active in immunized humans, which group comprises ATI locus proteins, A10L, A11R, A13L, A33R, A56R, B5R, D8L, D13L, F13L, H3L, H5R, A26L, A27L, E3L, and L4R.
[0285] Other immunologic compositions within the present invention are those which comprise at least three proteins that were found by the present method to be reactive in immunized humans, mice and macaques (all three species), which group comprises A10L, A11R, A13L, A33R, A56R, B5R, D8L, D13L, F13L, H3L, and HSR. Another immunologic composition within the present invention comprises at least one protein selected from the group of antigens most consistently recognized by various immunized individuals, which group includes ATI locus proteins, A10L, A13L, H3L, D13L, A11R, and A17R. And based on an overall impression of the strength and consistency of responses, the types of proteins, and similar considerations, another preferred immunologic composition within the present invention comprises at least two, or more preferably at least three, of the following vaccinia proteins: ATI locus proteins, A10L, A13L, A26L, A56R, D8L, D13L, F13L, HSR, and H3L.
[0286] Preferred compositions within the present invention include those comprising at least two proteins selected from the group consisting of ATI locus proteins, A10L, D13L, and H3L. Other preferred immunologic compositions comprise one of the consistently immunoactive proteins or peptides or substantially homologous forms or immunoactive fragments thereof selected from the group consisting of A10L, D13L, H3L, and ATI locus proteins in combination with an additional vaccinia antigen. Thus, for example, particularly preferred combinations would include those which combine H3L (or its substantial homologs or immunoactive fragments) with an additional immunogenic vaccinia protein. Another such combination would comprise a protein encoded by the ATI locus or a substantial homolog or immunoactive fragment thereof with an additional immunogenic vaccinia protein. Yet another embodiment comprises at least one protein selected from the group of novel antigens comprising A11R, A23L, A56R, and HSR, or one of these antigens in combination with at least one other antigenic vaccinia protein.
[0287] For each of the foregoing vaccine compositions, the invention also includes the corresponding DNA vaccines. Thus for each group of proteins set forth herein, a vaccine composition comprising the group of genes corresponding to the specified proteins is also within the scope of the invention as are the corresponding combinations of such genes with the corresponding vaccinia antigenic protein genes.
[0288] Thus the methodology identifies novel immunologically reactive antigens, not all of which would be identified by conventional predictive approaches. Data obtained with the arrays are in agreement with immunoblots we have reported previously, Crotty, S., et al., J. Immunol. (2003) 171:4969-4973, which is incorporated herein in its entirety by reference. Notably in vaccinated humans, we see strong anamnestic responses to a subset of dominant antigens after boosting many years after the primary immunization, notably to the H3L, D13L and A10L proteins.
EXAMPLE 7
Comparison of Protein Expression Using Plasmids Isolated From Single Colony/Clone or from Mixture of Transformation Culture
[0289] Twenty-eight (28) target genes ranging from 300 bp to 2000 bp in size from F. tularensis were selected and amplified by PCR using primers that contain 20 bp gene-specific sequence and 30 bp adaptor sequence homologous to corresponding ends of linear pIX expression vector (conferring T7 promoter and N-terminal poly-histidine fusion), as described above.
[0290] Twenty-five (25) ng of PCR product was pre-mixed with the same amount oflinear piX prep. The DNA mixture was transformed into 50 l chemically competent E. coli DH5a cells, left on ice for 30 minutes, heat-shocked for 45 seconds at 45 C., and mixed with 500 l of SOC media followed by incubation at 37 C. After 1 hour, 500 l of LB media containing Kanamycin (50 g/ml) was added followed by continuous incubation at 37 C. with shaking for >14-24 hours.
[0291] For single clone procedure, 50 l of the culture was then plated onto a LB agar plates with Kanamycin selection (25 g/ml) and incubated again at 37 C. for 12-14 hours. A single colony was then picked and cultured again overnight using the same media followed by DNA isolation using Qiagen miniprep kit.
[0292] Alternatively, plasmid DNA was isolated directly from the overnight transformation mixture in the first step, above.
[0293] The plasmid DNA (5 l) from steps 2 and 3 was added to 20 l Roche RTS 100 cell-free transcription/translation mix and incubated at 30 C. for 4 hours. 0.5 l of the expression mixture was spotted onto a nitrocellulose membrane followed by standard Western blot detection of the expressed protein using anti-poly-histidine tag monoclonal antibody.
Table 2
Protein Expression From Single Clone and Transformation Mixture (Results Showing Difference Between the Two Methods are Highlighted in Red Color)
[0294] Gene Name Expression of his-tag fusion [0295] Single colony Mixed culture [0296] #1788 [0297] #884 [0298] #1532 [0299] #558 [0300] #267 [0301] #226 [0302] #1148 [0303] #401 [0304] #316 [0305] #513 [0306] #617 [0307] #619 [0308] #397 [0309] #1894 [0310] Gene Name Expression of his-tag fusion [0311] Single colony Mixed culture [0312] #968 [0313] #257 [0314] #344 [0315] #1101 [0316] #570 [0317] #318 [0318] #352 [0319] #1531 [0320] #1056 [0321] #1167 [0322] #661 [0323] #2009 [0324] #1437 [0325] #1819
[0326] Single clone: 18 out 28 samples showed expression of the target gene. 10 samples did not give rise to any detectable level of protein expression.
[0327] Transformation mixture: 23 out of 28 samples showed expression. Five out of 10 negative samples from single clone protocol showed expression indicating plasmids from the single colonies may contain mutation(s) that prevented encoded protein from being expressed.
EXAMPLE 8
H3L Epitope Scan
[0328] The vaccinia envelope protein H3L was divided into 10 overlapping segments of 50 amino acids as shown in
[0329] To PCR amplify each segment, vaccinia genomic DNA was mixed with 10 M of the specific forward and reverse primers, water and Eppendorf HotMaster Mix to a final volume of 50 l. For 30 cycles, denaturation took place at 94 C. for 30 sec, followed by annealing at 50 C. for 30 sec and extension at 68 C. for 30 sec. After PCR, the products were run on a 1% agarose gel to assess the success of amplification. One gel showed enough products of segments 1, 2, and 6, a scanned gel showed enough of 3, 4, 8, and 10, and a third gel showed enough of 9. None of the PCR reactions successfully amplified segments 5 and 7. Therefore, instead of amplifying these two 150 bp segments, forward and reverse primers of 4 and 6 respectively were used to amplify 5, and forward and reverse primers of 6 and 8 were used to amplify 7. The amplification of these 450 bp sequences was successful.
[0330] After PCR amplification and cleanup of the PCR product using Qiagen PCR Purification Kit, the segments were cloned using recombination cloning. 40 ng of linearized pXi vector was mixed with 10 ng of cleaned up PCR product and to this mixture, 10 l of DH5 alpha E. coli competent cells was added. The mixture was then placed on ice for 45 minutes, heat shocked at 42 C. for 1 minute and then moved back to the ice for another minute. The mixture was removed and 200 l of SOC media was added to each tube and the mixture incubated in a 37 C. water bath for 1 hour. The transformation mixture was mixed with 3 mL of LB+Kanamycin and incubated overnight at 37 C.
[0331] Plasmid DNA was isolated from the transformation mixture using miniprep. Gels were run to determine if the plasmid had the insert. As a control, circular pXi vector was run. The results show that plasmids designed to contain segments 1, 2, 3, 6, 8, 9, and 10 had insert.
TABLE-US-00002 TABLE3 H3LPrimers Fragment DNAsequence FP(5-3) RP(5-3) (1) ATGGCGGCGGCGAAAACTCCTGTTATTGTTGTG CATATCGACGACGACGAC CATATCGACGACGACGAC CCAGTTATTGATAGACTTCCATCAGAAACATTT AAGCATATGCTCGAGATG AAGCATATGCTCGAGATG CCTAATGTTCATGAGCATATTAATGATCAGAAG GCGGCGGCGAAAACTCC GCGGCGGCGAAAACTCC TTCGATGATGTAAAGGACAACGAAGTTATGCCA GAAAAAAGAAATGTTGTG (2) GATCAGAAGTTCGATGATGTAAAGGACAACGAA CATACTCACGACGACGAC ATCTTAAGCGTAATCCGG GTTATGCCAGAAAAAAGAAATGTTGTGGTAGTC AAGCATATGCTCGAGGAT AACATCGTATGGGTAGGT AAGGATGATCCAGATCATTACAAGGATTATGCG CAGAAGTTCGATGATGT GAGTATACTTGTCATCAT TTTATACAGTGGACTGGAGGAAACATTAGAAAT GATGACAAGTATACTCAC (3) GATTATGCGTTTATACAGTGGACTGGAGGAAAC CATATCGACGACGACGAC ATCTTAAGCGTAATCCGG ATTAGAAATGATGACAAGTATACTCACTTCTTT AAGCATATGCTCGAGGAT AACATCGTATGGGTAGAA TCAGGGTTTTGTAACACTATGTGTACAGAGGAA TATGCGTTTATACAGTG AAAAATTAGAATAGAAAC ACGAAAAGAAATATCGCTAGACATTTAGCCCTA G TGGGATTCTAATTTTTTT (4)_ ACAGAGGAAACGAAAAGAAATATCGCTAGACAT CATATCGACGACGACGAC ATCTTAAGCGTAATCCGG TTAGCCCTATGGGATTCTAATTTTTTTACCGAG CTCGAGACAGAGGAAACG AACATCGTATGGGTAGCA TTAGAAAATAAAAAGGTAGAATATGTAGTTATT AAAAGAAA AGCCATTACAAGCTCGG GTAGAAAACGATAACGTTATTGAGGATATTACG TTTCTTCGTCCCGTCTTG (5) GTAGTTATTGTAGAAAACGATAACGTTATTGAG CATATCGACGACGACGAC ATCTTAAGCGTAATCCGG GATATTACGGCAATGCATGACAAAAAATAGATA AAGCATATGCTCGAGGTA AACATCGTATGGGTAGTT TCCTACAGATGAGAGAAATTATTACAGGCAATA GTTATTGTAGAAAACGA TGTCCATTACAAGCTCGG AAGTTAAAACCGAGCTTGTAATGGACAAA (6) CTACAGATGAGAGAAATTATTACAGGCAATAAA CATATCGACGACGACGAC ATCTTAAGCGTAATCCGG GTTAAAACCGAGCTTGTAATGGACAAAAATCAT AAGCATATGCTCGAGCTA AACATCGTATGGGTAGAT GCCATATTCACATATACAGGAGGGTATGATGTT CAGATGAGAGAAATTAT CTACGATGTTCAGCGCCG AGCTTATCAGCCTATATTATTAGAGTTACTACG GCGCTGAACATCGTAGAT (7) TATGATGTTAGCTTATCAGCCTATATTATTAGA CATATCGACGACGACGAC ATCTTAAGCGTAATCCGG GTTACTACGGCGCTGAACATCGTAGATGAAATT AAGCATATGCTCGAGTAT AACATCGTATGGGTAGCA ATAAAGTCTGGAGGTCTATCATCGGGATTTTAT GATGTTAGCTTATCAGC GTATCTGCCTATTGATCT TTTGAAATAGCCAGAATTGAAAACGAAATGAAG ATCAATAGGCAGATACTG (8) GGATTTTATTTTGAAATAGCCAGAATTGAAAAC CATATCGACGACGACGAC ATCTTAAGCGTAATCCGG GAAATGAAGATCAATAGGCAGATACTGGATAAT AAGCATATGCTCGAGGGA AACATCGTATGGGTAGTA GCCGCCAAATATGTAGAACACGATCCCCGACTT TTTTATTTTGAAATAGC TTCTAGACCAAAAATTCG GTTGCAGAACACCGTTTCGAAAACATGAAACCG AATTTTTGGTCTAGAATA (9) CCCCGACTTGTTGCAGAACACCGTTTCGAAAAC CATATCGACGACGACGAC ATCTTAAGCGTAATCCGG ATGAAACCGAATTTTTGGTCTAGAATAGGAACG AAGCATATGCTCGAGCCC AACATCGTATGGGTAGAA GCAGCTACTAAACGTTATCCAGGAGTTATGTAC CGACTTGTTGCAGAACA CATTAATATCAAACAATC GCGTTTACTACTCCACTGATTTCATTTTTTGGA TTGTTTGATATTAATGTT (10) GTTATGTACGCGTTTACTACTCCACTGATTTCA CATATCGACGACGACGAC ATCTTAAGCGTAATCCGG TTTTTTGGATTGTTTGATATTAATGTTATAGGT AAGCATATGCTCGAGGTT AACATCGTATGGGTAGTT TTGATTGTAATTTTGTTTATTATGTTTATGCTC ATGTACGCCTTTACTAC AGATAAATGCGGTAACGA ATCTTTAACGTTAAATCTAAACTGTTATGGTTC CTTACAGGAACATTCGTTACCGCATTTATCTAA
EXAMPLE 9
Detection of T-Cell Activation Using Proteins Immobilized on Beads
[0332] Using the methods described above, substantially all of the proteome of the organism in question (e.g. vaccinia) is cloned using a T7 vector (pTX7) and the proteins are expressed using a cell-free in vitro system. The adapter used to insert each protein into the vector includes a poly-His tag so the expressed proteins can be captured onto 1 m nickel-coated beads that have been previously equilibrated in a loading buffer (300 mM NaCl, 50 mM sodium phosphate 10 mM imidazole, pH 8.0). The nickel-coated beads may be of various sizes but are advantageously smaller than the APC cells, which are typically about 10-20 microns in diameter; nickel-coated beads that are 1-3 microns in size are available and sufficient for this purpose. The protein-coated beads are then washed 5 times in washing buffer (as above except with 20 mM imidazole), twice in tissue culture medium, and then resuspended in serum free medium to the original 12.5 l volume. These beads are incubated with antigen presenting cells prior to combining with T cells in 96 well assay format.
[0333] Responder T cells are obtained from mice immunized with the pathogen (e.g., 210.sup.5 pfu vaccinia administered intraperitoneally) or with individual recombinant proteins in adjuvant administered i.p. or subcutaneously at the base of the tail, or from the peripheral blood of infected/immunized human donors. In the case of mice, spleens or draining lymph nodes are removed 7-10d after immunization. Antigen-coated beads (usually 1-5 l per well) are then added to murine splenocytes or human peripheral blood mononuclear cells (PBMC; 510.sup.5 cells/well) in Multiscreen 96 well plates (Millipore MAHAS45) precoated with (from Pharmingen) and blocked for 1 h in tissue culture medium containing 10% fetal calf serum (FCS) (murine assays) or 5% human AB serum (human assays). The anti-mouse or human IFN- may be fixed into the well on a nitrocellulose substrate, for example; in that case, the treatment with serum serves to block any unoccupied sites on the nitrocellulose that could otherwise bind the capture antibody and interfere with the ELISPOT assay used to detect interferon or other cytokines formed. The IFN- antibodies capture any IFN- produced when the T-cells (splenocytes or PBMC) are stimulated by a recognized antigen. Thus after rinsing away unbound materials, any IFN- formed remains bound to the IFN- capture antibodies and is detected by addition of a second antibody capable of binding to the bound IFN-. This second antibody is labeled for easy visualization.
[0334] The medium used may be Iscove's Modified Dulbecco's Medium (IMDM) with Penicillin/Streptomycin/Glutamine and supplemented with 10-SOJ.Lg/ml polymyxin B to inhibit any contaminating LPS. For murine T cell assays, the medium is also supplemented with 2-mercaptoethanol to a final concentration of 510.sup.5 M. Positive control antigens for human assays may include tetanus toxoid, adsorbed onto alum (Colorado Serum Co) used at 1/160 and in TB-vaccinated donors, purified protein derivative (Tubersol from Aventis Pasteur). Mitogens that can be used to confirm assay and cell viability include Concanavalin-A for mouse cells and phytohemagglutinin for human cells, both used at 1 g/ml. Antibodies for IFN- detection by ELISPOT are matched pairs from Pharmingen.
[0335] After 18 to 20 h of co-cultivation, captured interferon is detected with biotinylated anti-IFN- detection antibody (Pharmingen) and visualized with streptavidin-alkaline phosphatase followed by nitro-BT developer. Supernatants of human and murine cultures are also taken at 6 h, 12 h, 24 h and 48 h and subjected to multiplex cytokine analysis (using custom 10-plex kits from Linco Research Inc) for Thl (IFN-, TNF-, and IL-12) Th2 (IL-4, IL-6, IL-10 and IL-13) and inflammatory cytokines (IL-1, IL-2 and GM-CSF) and maybe analyzed simultaneously using a Luminex 100 machine. The presence of one or more of these cytokines demonstrates that the protein being tested elicits a cellular immune response, and allows one to identify those proteins or peptides useful for eliciting immunity.
EXAMPLE 10
Detection Off-Cell Activation Using Expression of Proteins in APCs
[0336] Substantially all of the proteome of the organism in question (e.g. vaccinia) is cloned into the CMV (gWIZ) vector. Plasmids are introduced in antigen presenting cells (APCs) using lipid delivery (by Lipofection, using special lipid reagents such as Lipofectin from Invitrogen, Cytofectene Transfection Reagent by Bio-Rad, or FuGENE 6 Transfection Reagent by Roche Applied Science; see Feigner, et al., Proc. Nat'l. Acad. Sci. USA., November 1987 84(21), 7413-7, which is incorporated herein in its entirety by reference) after 1 day, to allow the proteins to be expressed prior to combining with T cells in 96 well assay format. Responder T cells are obtained from mice immunized with the pathogen (e.g., 210.sup.5 pfu vaccinia administered intraperitoneally) or with individual recombinant proteins in adjuvant administered i.p. or subcutaneously at the base of the tail, or from the peripheral blood of infected/immunized human donors. In the case of mice, spleens or draining lymph nodes are removed 7-10 days after immunization. Transfected antigen presenting cells are then added to murine splenocytes or human PBMC (510.sup.5 cells/well) in Multiscreen 96 well plates (Millipore MAHAS45) precoated with anti-mouse or human IFN-Y (from Pharmingen) and blocked for 1 h in tissue culture medium containing 10% FCS (murine assays) or 5% human AB serum (human assays).
[0337] The medium used may be Iscove's Modified Dulbecco's Medium (IMDM) with Penicillin/Streptomycin/Glutamine and supplemented with 10-50 g/ml polymyxin B to inhibit any contaminating LPS (lipopolysaccharides). For murine T cell assays, medium is also supplemented with 2-mercaptoethanol to a final concentration of 510.sup.5M. Positive control antigens for human assays may include tetanus toxoid, adsorbed onto alum (Colorado Serum Co) used at 1/160 and in TB-vaccinated donors, purified protein derivative (Tubersol from Aventis Pasteur). Mitogens to confirm assay and cell viability can include Concanavalin-A for mouse cells and phytohemagglutinin for human cells, each of which is used at 1 g/ml. Antibodies for IFN- detection by ELISPOT are matched pairs from Pharmingen.
[0338] After 18 to 20 h of co-cultivation, captured interferon is detected with biotinylated anti-IFN- detection antibody (Pharmingen) and visualized with streptavidin-alkaline phosphatase followed by nitro-BT developer. Supernatants of human and murine cultures are also taken at 6 h, 12 h, 24 h and 48 h and subjected to multiplex cytokine analysis (using custom 10-plex kits from Linco Research Inc) for Thl (IFN-, TNF-, and IL-12) Th2 (IL-4, IL-6, IL-10 and IL-13) and inflammatory cytokines (IL-1, IL-2 and GM-CSF) and maybe analyzed simultaneously using a Luminex 100 machine. The presence of one or more of these cytokines demonstrates that the protein being tested elicits a cellular immune response, and allows one to identify those proteins or peptides useful for eliciting immunity.
EXAMPLE 11
Validation of the Antigen Identification Method Using Malaria (P. (alciparum)
[0339] A set of 218 P.falciparum (Pf) genes were selected for cloning, expression, and protein microarray chip printing. The genes were selected on the basis of subcellular localization (e.g., secreted proteins and other proteins found in cell culture supernatants), known immunogenicity in human and animal models of P. falciparum, and pattern of gene expression vis-a-vis Plasmodium growth state. Each fit into one of nine categories: i) Identified by bioinformatic criteria only (n=25); ii) Identified by laser capture microdissection of P. yoelii liver-stages, and identified in sporozoite proteome by MudPIT (n=16); iii) Pf orthologues of proteins identified by laser capture microdissection ofPy liver-stage but not found in sporozoite proteome (liver-stage specific; n=52); iv) Highly expressed in sporozoite proteome by MudPIT (n=10); v) Identified in sporozoite proteome by MudPIT and assayed for immune recognition by PBMCs from irradiated sporozoite (irr-spz) immunized volunteers (n=27); vi) Known and well characterized Pf antigens in clinical development (n-21); vii) Highly expressed in sporozoite stage as evidenced by gene transcript profiling of sporozoites by Affymetrix gene chips (n=53); viii) Identified in trophozoite and schizont-stage proteome by MudPIT (n=11); and ix) P. falciparum orthologues of P. yoelii antigens indicated to be protective in vivo (n=2). One additional gene of interest that was included, PFB0645c, does not fit into any of these categories.
[0340] PCR amplification was accomplished using P. falciparum genomic DNA template. Since many P. falciparum genes contain introns, primers were designed to span each exon. Large genes (and exons) greater than 3000 base pairs were amplified in segments with each segment overlapping by 150 nucleotides (i.e. 50 amino acids). Primer design covering the entire P. falciparum genome was done by Arlo Randall at the Institute of Genomics and Bioinformatics at UC Irvine and the primer database is accessible through a Web interface. The database contains 14,446 entities. Thus to amplify each independent exon and to amplify large genes in segments less than 3000 bp would require 14,446 primer pairs. However, about 40% of the ORFs encode short peptides less than 50 amino acids, so about 8000 primer pairs would be required to amplify each ORF greater than 150 nucleotides. This on-line database was used as the source of primer sequences for the following study.
[0341] A total of 266 ORFs derived from the 218 gene target set were amplified, cloned, and expressed using the expressions system previously described. Using a process that took 3 days to complete, 266 ORFs were PCR amplified from P. falciparum genomic DNA, the fragments were cloned into a T7 expression vector, expressed in a cell-free in vitro transcription/translation system and the expressed proteins were spotted onto microarray chips. The chips were probed with E. coli lysate treated sera from irradiated sporozoite immunized human volunteers, the slides were developed with Cy3 labeled anti-human antibody and read with a laser confocal microarray chip reader. The malaria immune individuals reacted against a subset of P. falciparum proteins, whereas naive individuals were not reactive. The proteins were printed onto microarray chips, and the chips were probed with sera from 11 donors who were naturally exposed to malaria in hyperendemic region of Kenya, or had been immunized with irradiated sporozoites. Naive donors lacked reactivity against the complete set of expressed proteins printed on the chip (
[0342] There were 9 strongly reactive proteins identified from this analysis. Seven out of the nine highly reactive proteins are known, well characterized Pf blood-stage antigens, many of which are under clinical development and evaluation (LSA3, MSP4, EBA175, RESA). Interestingly, PF10_0356, Liver Stage Antigen 1, is a liver-stage specific antigen; it is NOT expressed in the sporozoite or blood-stages of the organism, only in the liver stage. So the fact that 6 of 11 sera recognized this antigen demonstrates that the proteome arrays have the capacity to identify more than just the blood stage antigens. Also, PFD031Ow is SHEBA/Pfs16, a sexual stage antigen under clinical development as a vaccine antigen candidate. One of the most strongly reactive antigens, PFE1590w has not been previously recognized as a potential vaccine antigen candidate.
TABLE-US-00003 TABLE 4 Serum Reactivity in Malaria Immune Subjects. #of Responders Gene Locus Protein ID 11 PFB0300c merozoite surface protein 2 precursor (MSP2) 11 PFB0915w* liver stage antigen 3 (LSA3) 10 PFB0310c* merozoite surface protein 4 (MSP4) 9 PFE1590w early transcribed membrane protein 8 PFD0310w sexual stage-specific protein precursor (SHEBA/Pfs16) 6 PF07_0128 erythrocyte binding antigen (EBA175) 6 PF10_0343* S-antigen 6 PF10_0356 liver stage antigen, putative (LSA1) 6 PF11_0509* ring-infected erythrocyte surface antigen (RESA) *These genes included introns, and were expressed as two separate proteins, overlapping by 20 amino acids. At least one of the two proteins is antigenic.
[0343] By way of example only and without limiting the scope of proteins or DNA sequences encompassed by the invention, some of the closest orthologs for some of the immunoactive proteins identified by the present method, some of which are not in Table 4, include:
[0344] PFB0310c:
[0345] P. yoelii: PY05967 (MSP4/5 related)
[0346] P. yoelii: PY07543 (MSP 4/5)
[0347] PFE1590w:
[0348] P. yoelii: PY02667 (integral membrane protein)
[0349] PFB07 0128:
[0350] P. falciparum: Chr. 13, MAL13P1.60 (erythrocyte binding antigen 140)
[0351] P. falciparum Chr. 1, PFA0125c (Ebl-11ike protein, putative)
[0352] P. falciparum Chr. 1, PFA0065w (hypothetical protein)
[0353] P. falciparum Chr. 4, PFD1155w (erythrocyte binding antigen, putative)
[0354] P. yoelii PY04764 (duffy receptor, beta form precursor)
[0355] PF10 0343:
[0356] P. yoellii PY04926 (hypothetical protein)
[0357] PF11 0509:
TABLE-US-00004 gene species description MAL6P1.19 P. falciparum hypothetical protein MAL7P1.174 P. falciparum hypothetical protein MAL7P1.7 P. falciparum RESA-like protein MAL8P1.2 P. falciparum hypothetical protein with DNAJ domain PF10_0378 P. falciparum hypothetical protein PF11_0037 P. falciparum hypothetical protein PF11_0509 P. falciparum ring-infected erythrocyte surface antigen, putative PF11_0512 P. falciparum ring-infected erythrocyte surface antigen 2, RESA-2-malaria parasite (Plasmodium falciparum)-related PF11_0513 P. falciparum hypothetical protein PF14_0018 P. falciparum hypothetical protein PF14_0732 P. falciparum hypothetical protein PF14_0746 P. falciparum hypothetical protein PFA0110w P. falciparum ring-infected erythrocyte surface antigen precursor PFB0080c P. falciparum hypothetical protein PFB0085c P. falciparum hypothetical protein PFB0920w P. falciparum hypothetical protein PFD0095c P. falciparum hypothetical protein PFD1170c P. falciparum hypothetical protein PFD1180w P. falciparum Plasmodium falciparum trophozoite antigen-like protein PFE1600w P. falciparum hypothetical protein PFE1605w P. falciparum protein with DNAJ domain PFI0130c P. falciparum hypothetical protein PFI1785w P. falciparum hypothetical protein PFI1790w P. falciparum hypothetical protein PFL0055c P. falciparum protein with DNAJ domain (resa-like), putative PFL2535w P. falciparum RESA-like protein, putative PFL2540w P. falciparum hypothetical protein
[0358] PF13 0197:
[0359] P. falciparum: CHR 13/MAL13P1.173/MSP7-like protein
[0360] P. falciparum: CHR 13/MAL13P1.174/MSP7-likeprotein
[0361] P.falciparum: CHR 13/PF13_0193/MSP7-like protein
[0362] P.falciparum: CHR 13/PF13_0196/MSP7-like protein
[0363] P.falciparum: CHR 13/PF13_0197/Merozoite Surface Protein 7 precursor,
[0364] MSP7
[0365] P. yoelii: PY02147/Meloidogyne incognita COL-1-related
[0366] PF14_0486:
[0367] P. yoelii PY05356 (elongation factor 2)
[0368] PF08_0054:
[0369] P.yoelii PY06158 (heat shock protein 70)
[0370] PF11_0344:
[0371] P. yoelii PY01581 (apical membrane antigen-1)
[0372] In a separate application of these methods, 300 genes from P. falciparum were expressed and displayed in a microarray using the methods described herein. The array was probed with serum from 12 subjects who contracted malaria at an early age and were thus immunized to it. Positive responses were observed in at least six of the twelve serum samples for each of the following gene products:
TABLE-US-00005 TABLE 4b Serum Reactivity in Malaria Immune Subjects. Genes Positive (Locus tag responses used in GenBank) Description from GenBank (out of 12 sera) PFB0915w LSA-3-e2s1 12 PFB0310c MSP-4-e1 12 PFB0300c MSP-2 12 PFB0305c MSP-5-e1 12 PFL2410w hypothetical protein-e1 12 PFC0210c Circumsporozoite (CS) prot 12 PFD0310w sex stg-spec prot prec a 11 PFD0310w sex stg-spec prot prec b 11 PF13_0197 MSP7 precursor 11 PF10_0138 hypothetical prot-s1 11 PFI1520w hypothetical protein b 11 PFI1520w hypothetical protein a 11 PF11_0344 ap memb antigen 1 prec 11 PF13_0012 hypothetical prot 10 PFD0310w sex stg-spec prot prec 10 PF11_0358 DNA-dir RNAP, B subunit-e1 10 PF07_0029 HSP86-e1 10 PFL1605w hypothetical prot-s2 10 PFE1590w early transc memb prot 10 MAL6P1.201 leucyl-trna synthetase, 10 cytoplasmic-s2 PFD0235c hypothetical prot-e1 9 PF13_0201 spz surf prot 2 9 PF13_0267 hypothetical protein a 9 PF07_0128 erythrocyte binding antigen-e1s2 9 PF10_0343 S-Antigen a 9 PF10_0343 S-Antigen 9 PFI1520w hypothetical protein 8 PFI0580c Hypo Asn-rich prot w/N-term sig 8 seq-e2 PF07_0020 hypothetical prot-e1s2 8 PFE0520c topoisomerase I 8 MAL7P1.29 hypothetical protein-e1s2 8 PF10_0260 hypothetical protein-e2s2 8 PF11_0358 DNA-dir RNAP, B subunit-e2s2 7 MAL8P1.139 hypothetical prot-e3 7 PF13_0228 PF01092 Rib prot S6e 7 PF10_0132 phospholipase C-like-e1s2 7 PFB0855c hypothetical prot-e2 7 PF10_0125 hypothetical prot 7 PF13_0350 SRP54-type prot, GTPase dam 7 PFD0665c-e2 7 MAL7P1.32 hypothetical prot 7 PF07_0016 hypothetical prot-s1 7 PF10_0098a 6 PF08_0056 zinc finger protein-e2 6 PFB0640c-e1s1 6 PF14_0230 Rib prot fam L5-e2 6 PF14_0315 hypothetical prot-e2s1 6 PF08_0088 hypothetical prot 6 PFL0685w hypothetical prot-e2 6 MAL7P1.23 hypothetical prot-e1s2 6 PFE0060w hypothetical prot-e2 6 MAL8P1.23 ubiquitin-prot ligase 1-s8 6 PF07_0029 HSP86-e2 6 PF10_0356 LSA-e2s2 6
EXAMPLE 12
Malaria Vaccines and Diagnostic Tests
[0373] From the data set obtained in Example 11, a cocktail of proteins or nucleic acids encoding proteins is selected for a vaccine composition. A malaria vaccine cocktail based on these results comprises at least three of the following genes or the corresponding peptides, and four or more, or five or more, or it may include all of these: PFB0300c, PFE1590w, PFB0915w, PFB0310c, PFB0310w, PF11_0509, and PF10_0343. This vaccine is administered using the excipients, compositions and methods disclosed herein to immunize a human subject at risk for malaria, provided the subject's immune system is not compromised.
[0374] Alternatively, a vaccine would comprise at least three of the nucleic acids or three of the proteins corresponding to the genes identified in Table 4b as ones expressing antigenic proteins. In a preferred embodiment, the vaccine would comprise more than three or more than four or at least six of these proteins or nucleic acids. Typically, the vaccine wouldcomprise at least three nucleic acids or proteins corresponding to the genes whose gene product gave a positive response in at least six of the tested sera, or in at least 8 of the tested sera; or in at least 9 of the tested sera; or in at least 10 of the tested sera; or in at least 11 of the tested sera. In some embodiments, the vaccine would comprise at least one component corresponding to one of the genes that elicited a positive response in 10 or more of the sera tested. In other embodiments, the vaccine would comprise at least two protein or nucleic acid components or at least three protein or nucleic acid components corresponding to genes that elicited a positive response in 10 or more of the 12 sera tested. In other embodiments the immunodomiant antigens would be used in a serological diagnostic test, such as ELISA, to unambiguously diagnose whether a person has be exposed or infected by P. falciparum.
EXAMPLE 13
Antigenic Proteins Identified in Francisella Tularensis
[0375] Following the methods described above using the proteins of Example 1D from F. tularensis, a number of antigenic proteins were identified that were reactive with serum from mice that were exposed to a non-infectious strain of Francisella or from mice that were exposed to the virulent Schu S4 strain. Data for those proteins is in Tables 5 and 6 below. The sequences for the proteins are available in the GenBank database, which is available online at the web address www.ncbi.nlm.nih.gov/gquery/gquery.fcgi. The gene code in the table corresponds to the locus tag for the gene and protein identified.
TABLE-US-00006 TABLE 5 Antigens detected with serum from mice exposed to non-infectious strain. Mice exposed to non-infectious strain (each col. Represents 5-6 mice) Proteins Genes 1 to 6 7 to 12 13 to 17 18 to 22 DnaK (HSP70) FTT1269 x x x TM protein (OmpH) FTT1747 x x x x HSP60 (Cpn60) FTT1696 x x TM protein FTT0975 x x x 17 kd Protein (IpnA) FTT0901 FTT0901 x x FTT1477 biotin carboxyl FTT0472 x x carrier FTT0264
TABLE-US-00007 TABLE 6 Antigenic proteins detected by serum from mice challenged with Schu 84. Murine Schus4 challenge Mice Pools (each col. Represents serum from 5-6 mice) Proteins Genes 1 to 6 7 to 12 13 to 17 18 to 22 DnaK (HSP70) FTT1269 x x x x TM protein (OmpH) FTT1747 x x x x HSP60 (Cpn60) FTT1696 x x x x 1272 SS TM protein FTT0975 x x x 17 kd Protein (IpnA) FTT0901 x FTT0901 x FTT1477 x x biotin carboxyl carrier FTT0472 x FTT0264 x
[0376] The tables show that the mice challenged with a virulent organism produced more antibodies than those challenged only with the non-infectious strain, and that certain antibodies were produced very consistently regardless of which strain was used to immunize the mice.
[0377] By way of example only and without limiting the scope of proteins or DNA sequences encompassed by the invention, some of the closest variants and orthologs for some of the immunoactive proteins identified by the present method include:
[0378] FTT1269 (DnaK): [0379] Pseudomonas aeruginosa PAO1 [0380] Pseudomonas putida KT2440 [0381] Legionella pneumophila [0382] Coxiella bumetii strain RSA 493 [0383] Legionella pneumophila str. Lens [0384] Legionella pneumophila str. Paris [0385] Coxiella bumetii dnaK [0386] Legionella pneumophila grpE, dnaK, dnaJ [0387] Salmonella enterica [0388] Salmonella enterica serovar Typhi (Salmonella typhi) strain CT18
[0389] FTT1696 (Hsp60): [0390] Acinetobacter sp. ADP1 [0391] Xenorhabdus nematophila GroEL-like protein gene [0392] Vibrio cholerae O1 biovar eltor str. N16961 chromosome I [0393] Pseudomonas aeruginosa PAO1 [0394] Klebsiella pneumoniae gene for GroES protein homologue, GroEL protein homologue [0395] Enterobacter agglomerans gene for GroES protein homologue, GroEL protein homologue [0396] Enterobacter asburiae gene for GroES protein homologue, GroEL protein homologue [0397] Pseudomonas aeruginosa GroEL (mopA) gene [0398] Enterobacter aerogenes gene for GroES protein homologue, GroEL protein homologue [0399] Pseudoalteromonas sp. PS1M3 gene for GroES, GroEL
[0400] FTT0901 (17 kd protein): [0401] Francisella endosymbiont of Dennacentor albipictus clone T1G 17 kDa lipoprotein gene [0402] Francisella endosymbiont of Dermacentor variabilis clone 01-109 17 kDa lipoprotein gene [0403] Francisella endosymbiont of Dermacentor occidentalis clone 02-241 17 kDa lipoprotein gene [0404] Francisella endosymbiont of Dermacentor hunteri clone 01-113 17 kDa lipoprotein gene [0405] Francisella endosymbiont of Dermacentor andersoni clone 01-151-1 17 kDa lipoprotein gene [0406] Francisella endosymbiont of Dermacentor andersoni clone 01-171 17 kDa lipoprotein gene [0407] Francisella endosymbiont of Dermacentor nitens clone DnT2-1 17 kDa lipoprotein gene [0408] Francisella endosymbiont of Dermacentor hunteri clone 02-249 17 kDa lipoprotein gene [0409] Francisella endosymbiont of Dermacentor hunteri clone 01-112 17 kDa lipoprotein gene [0410] Francisella endosymbiont of Dermacentor andersoni clone 02-31 17 kDa lipoprotein gene
[0411] FTT1477c: [0412] Pseudomonas putida KT2440 [0413] Pseudomonas syringae pv. tomato str. DC3000 [0414] Pseudomonas aeruginosa PA01 [0415] Xanthomonas axonopodis pv. citri str. 306 [0416] Xanthomonas campestris pv. campestris str. ATCC 33913 [0417] Photobacterium profundum SS9 [0418] Methylococcus capsulatus str. [0419] Bath Legionella pneumophila str. [0420] Paris Legionella pneumophila str. Lens [0421] Bradyrhizobium japonicum USDA 110
[0422] DNA [0202] FTT0472 (biotin carboxyl carrier): [0423] Pseudomonas aeruginosa PA01 [0424] Pseudomonas aeruginosa biotin carboxyl carrier protein and biotin [0425] carboxylase (accB and accC) genes [0426] Legionella pneumophila subsp. pneumophila str. Philadelphia 1 [0427] Legionella pneumophila str. Paris [0428] Pasteurella multocida subsp. multocida str. Pm70 [0429] Legionella pneumophila str. Lens [0430] Methylococcus capsulatus str. [0431] Bath Shigella flexneri 2a str. [0432] Salmonella typhimurium LT2 [0433] Shigella flexneri 2a str. 2457T
EXAMPLE 14
Antigenic Proteins from Mycobacterium Tuberculosis
[0434] Following the methods described above using the proteins of Example 1C from Mycobacterium tuberculosis H37Rv, the following antigenic proteins were identified (selected known variants and orthologs are also presented as non-limiting examples):
[0435] Rv3333c (hypothetical proline rich protein)
TABLE-US-00008 Variants/orthologs: Mb2765c (M. bovis) ML0981 (M. leprae)
[0436] Rv0440 (60 kDa chaperonin)
TABLE-US-00009 Variants/orthologs: Mb0448 (M. bovis) ML0317 (M. leprae)
[0437] Rv1860 (alanine and proline rich secreted protein APA)
TABLE-US-00010 Variants/orthologs: Mb1891 (M. bovis)
[0438] Rv3763 (19 kDa liproprotein antigen precursor LPQH)
TABLE-US-00011 Variants/orthologs: Mb3789 (M. bovis) ML1966 (M. leprae)
[0439] Rv3874 (10 kDa culture filtrate antigen ESXB)
TABLE-US-00012 Variants/orthologs: Mb2765c (M. bovis)
[0440] Rv3875 (6 kDa early secretory antigenic target ESXA)
TABLE-US-00013 Variants/orthologs: Mb3905 (M. bovis)
EXAMPLE 15
Antigenic Proteins from Mycobacterium Tuberculosis
[0441] Proteins from 312 expressed genes of Mycobacterium tuberculosis H37Rv were tested with sera from rabbits, mice, and monkeys using the methods described above and proteins from the genes obtained in Example 1C. The following table lists the antigens detected using serum from each species: each protein is identified by the locus tag for the corresponding gene that is used in the publicly available GenBank database. The serum of non-infected animals reacted to all of the antigens listed; the antigens that were only detected by serum from TB-infected animals are listed in boldface and highlighted.
TABLE-US-00014 TABLE 7 Rabbit Mouse Monkey Rv0040 Rv0040 Rv0440 Rv0292 Rv0102 Rv0475 Rv0432 Rv0292 Rv0577 Rv0674 Rv0366c Rv1801 Rv0867c Rv0432 Rv1860 Rv1004c Rv0440 Rv1980c Rv1157c Rv0467 Rv2220 Rv1184c Rv0526 Rv2744c Rv1310 Rv0538 Rv2873 Rv1435c Rv0545c Rv2875 Rv1620c Rv0685 Rv3270 Rv1733c Rv0798c Rv3333c Rv1801 Rv0847 Rv3418c Rv1837c Rv0886 Rv3763 Rv1860 Rv0916c Rv3873 Rv2031c Rv0934 Rv3874 Rv2190c Rv1004c Rv3875 Rv2195 Rv1244 Rv3875 & Rv3874 Fusion Rv2253 Rv1307 Rv3881c Rv2376c Rv1311 Rv2700 Rv1435c Rv2721c Rv1451 Rv2744c Rv1566c Rv2744c Rv1620c Rv2864c Rv1623c_1 Rv3270 Rv1686c Rv3333c Rv1733c Rv3449 Rv1737c Rv3873 Rv1860 Rv1906c Rv1926c Rv1984c Rv2007c Rv2031c Rv2193 Rv2195 Rv2196 Rv2253 Rv2376c Rv2389c Rv2446c Rv2495c Rv2620c Rv2700 Rv2744c Rv2873 Rv2875 Rv3217c Rv3270 Rv3330 Rv3333c Rv3390 Rv3418c Rv3524 Rv3705c Rv3714c Rv3803c Rv3828c Rv3841 Rv3846 Rv3873 Rv3874 Rv3875 Rv3881c Rv3914
EXAMPLE 16
Tuberculosis Vaccines and Diagnostic Tests
[0442] From the data set obtained in Example 15, a cocktail of proteins or nucleic acids encoding proteins is selected for a vaccine composition. A tuberculosis diagnostic test or vaccine cocktail based on these results comprises at least three of the following genes or the corresponding peptides, and may include four or more, or five or more, or most or all of these: Rv0440, Rv0467, Rv0475, Rv0538, Rv0674, Rv0685, Rv0798c, Rv0916c, Rv0934, Rv1801, Rv1860, Rv1926c, Rv1980c, Rv1984c, Rv2007c, Rv2031c, Rv2190c, Rv2220, Rv2376c, Rv2389c, Rv2446c, Rv2744c, Rv2873, Rv2875, Rv2875, Rv3270, Rv3330, Rv3333c, Rv3418c, Rv3763, Rv3803c, Rv3828c, Rv3846, Rv3874, Rv3875, Rv3881c, and Rv3914. Especially suitable antigens include those that were reactive specifically to semm from infected animals of multiple species, which include Rv0440, Rv1801, Rv2031c, Rv2376c, Rv2875, and Rv3875. Also of special interest are those antigens that were specifically recognized by serum from infected monkeys, including Rv0440, Rv0475, Rv1801, Rv1980c, Rv2220, Rv2873, Rv2875, Rv3270, Rv3763, and Rv3875. The vaccine or diagnostic test may therefore comprise two or more, or three or more, or more than three proteins or nucleic acids selected from either of these groups of antigens.
[0443] This vaccine is administered using the excipients, compositions and methods disclosed herein to immunize a human subject at risk for tuberculosis, provided the subject's immune system is not compromised.
TABLE-US-00015 TABLE 8 VACV-COP Locus Name Ortholog SIZE STRAND START FINISH VACWR129 A10L 891 121844 119169 VACWR130 A11R 318 + 121859 122815 VACWR131 A12L 192 123395 122817 VACWR132 A13L 70 123631 123419 VACWR133 A14L 90 124011 123739 VACWR135 A15L 94 124463 124179 VACWR136 A16L 377 125580 124447 VACWR137 A17L 203 126194 125583 VACWR138 A18R 493 + 126209 127690 VACWR139 A19L 77 127904 127671 VACWR119 A1L 150 110357 109905 VACWR141 A20R 426 + 128257 129537 VACWR140 A21L 117 128258 127905 VACWR142 A22R 187 + 129467 130030 VACWR143 A23R 382 + 130050 131198 VACWR144 A24R 1164 + 131195 134689 VACWR145 A25L 65 134891 134694 VACWR146 A26L-a 154 135324 134860 VACWR148 ATI locus proteinr 136239 138416 VACWR149 A26L-b 500 139963 138461 VACWR150 A27L 110 140345 140013 VACWR151 A28L 146 140786 140346 VACWR152 A29L 305 141704 140787 VACWR120 A2L 224 111052 110378 VACWR153 A30L 77 141900 141667 VACWR154 A31R 124 + 142060 142434 VACWR155 A32L 270 143213 142401 VACWR156 A33R 185 + 143331 143888 VACWR157 A34R 168 + 143912 144418 VACWR158 A35R 176 + 144462 144992 VACWR159 A36R 221 + 145059 145724 VACWR160 A37R 263 + 145788 146579 VACWR162 A38L 277 147687 146854 VACWR164 A39R 142 + 148474 148902 VACWR122 A3L 644 113228 111294 VACWR165 A40R 159 + 148928 149407 VACWR166 A41L 219 150164 149505 VACWR167 A42R 133 + 150328 150729 VACWR168 A43R 194 + 150767 151351 VACWR170 A44L 346 152733 151693 VACWR171 A45R 125 + 152780 153157 VACWR172 A46R 240 + 153147 153869 VACWR173 A47L 252 154675 153917 VACWR174 A48R 227 + 154706 155389 VACWR175 A49R 162 + 155437 155925 VACWR123 A4L 281 114126 113281 VACWR176 ASOR 552 + 155958 157616 VACWR177 A51R 334 + 157669 158673 VACWR178 A52R 190 + 158743 159315 VACWR179 A53R 103 + 159621 159932 VACWR180 A55R 564 + 160439 162133 VACWR181 A56R 314 + 162183 163127 VACWR182 A57R 151 + 163272 163727 VACWR124 ASR 164 + 114164 114658 VACWR125 A6L 372 115773 114655 VACWR126 A7L 710 117929 115797 VACWR127 ABR 288 + 117983 118849 VACWR128 A9L 108 119168 118842 VACWR192 B10R 166 + 171672 172172 VACWR193 B11R 72 + 172244 172462 VACWR194 B12R 283 + 172529 173380 VACWR195 B14R 345 + 173473 174510 VACWR196 B15R 149 + 174585 175034 VACWR197 B16R 326 + 175118 176098 VACWR198 B17L 340 177166 176144 VACWR199 B18R 574 + 177306 179030 VACWR203 B18R 309 + 180898 181827 VACWR200 B19R 351 + 179102 180157 VACWR183 B1R 300 + 163878 164780 VACWR202 B20R 53 + 180482 180643 VACWR184 B2R 219 + 164870 165529 VACWR185 B3R 167 + 165565 166068 VACWR186 B4R 558 + 166594 168270 VACWR187 BSR 317 + 168374 169327 VACWR188 B6R 173 + 169409 169930 VACWR189 B7R 182 + 169968 170516 VACWR190 BBR 272 + 170571 171389 VACWR191 B9R 77 + 171476 171709 VACWR209 C10L 331 + 185807 186802 VACWR210 C11R 140 187379 186957 VACWR205 C12L 353 + 182511 183572 VACWR206 C14L 190 + 183734 184306 VACWR017 C17L 71 12682 12467 VACWR008 C19L 112 7060 6722 VACWR027 C1L 229 21832 21143 VACWR212 C20L 109 + 188295 188624 VACWR006 C21L 64 6155 5961 VACWR004 C22L 122 5460 5092 VACWR001 C23L 244 4375 3641 VACWR026 C2L 512 21073 19535 VACWR025 C3L 263 19468 18677 VACWR024 C4L 316 18610 17660 VACWR023 C5L 204 17597 16983 VACWR022 C6L 151 16856 16401 VACWR021 C7L 150 16168 15716 VACWR020 C8L 177 15644 15111 VACWR019 C9L 634 15068 13164 VACWR115 D10R 248 + 104655 105401 VACWR116 D11L 631 107297 105402 VACWR117 D12L 287 108195 107332 VACWR118 D13L 551 109881 108226 VACWR106 D1R 844 + 93948 96482 VACWR107 D2L 146 96881 96441 VACWR108 D3R 237 + 96874 97587 VACWR109 D4R 218 + 97587 98243 VACWR110 D5R 785 + 98275 100632 VACWR111 D6R 637 + 100673 102586 VACWR112 D7R 161 + 102613 103098 VACWR113 D8L 304 103975 103061 VACWR114 D9R 213 + 104017 104658 VACWR066 E10R 95 + 56688 56975 VACWR067 E11L 129 57359 56970 VACWR057 E1L 479 45443 44004 VACWR058 E2L 737 47653 45440 VACWR059 E3L 190 48352 47780 VACWR060 E4L 259 49187 48408 VACWR061 ESR 341 + 49236 50261 VACWR062 E6R 567 + 50398 52101 VACWR063 E7R 166 + 52183 52683 VACWR064 ESR 273 + 52808 53629 VACWR065 E9L 1006 56656 53636 VACWR049 F10L 439 37778 36459 VACWR050 F11L 348 38847 37801 VACWR051 F12L 635 40797 38890 VACWR052 F13L 372 41949 40831 VACWR053 F14L 73 42188 41967 VACWR054 F15L 147 42903 42460 VACWR055 F16L 231 43639 42944 VACWR056 F17R 101 + 43702 44007 VACWR040 F1L 226 31026 30346 VACWR041 F2L 147 31481 31038 VACWR042 F3L 480 32947 31505 VACWR043 F4L 319 33917 32958 VACWR044 FSL 322 34917 33949 VACWR045 F6L 74 35171 34947 VACWR046 F7L 80 35429 35187 VACWR047 FSL 65 35774 35577 VACWR048 F9L 212 36472 35834 VACWR078 G1L 591 70752 68977 VACWR080 G2R 220 + 71078 71740 VACWR079 G3L 111 71084 70749 VACWR081 G4L 124 72084 71710 VACWR082 G5R 434 + 72087 73391 VACWR084 G6R 165 + 73592 74089 VACWR085 G7L 371 75169 74054 VACWR086 GSR 260 + 75200 75982 VACWR087 G9R 340 + 76002 77024 VACWR099 H1L 171 87737 87222 VACWR100 H2R 189 + 87751 88320 VACWR101 H3L 324 89297 88323 VACWR102 H4L 795 91685 89298 VACWR103 HSR 203 + 91871 92482 VACWR104 H6R 314 + 92483 93427 VACWR105 H7R 146 + 93464 93904 VACWR070 I1LL 312 60804 59866 VACWR071 I2L 73 61032 60811 VACWR072 I3L 269 61842 61033 VACWR073 I4L 771 64240 61925 VACWR074 I5L 79 64506 64267 VACWR075 I6L 382 65673 64525 VACWR076 I7L 423 66937 65666 VACWR077 I8R 676 + 66943 68973 VACWR093 J1R 153 + 80247 80708 VACWR094 J2R 177 + 80724 81257 VACWR095 J3R 333 + 81323 82324 VACWR096 J4R 185 + 82239 82796 VACWR097 JSL 133 83258 82857 VACWR098 J6R 1286 + 83365 87225 VACWR032 K1L 284 25925 25071 VACWR033 K2L 369 27256 26147 VACWR034 K3L 88 27572 27306 VACWR035 K4L 424 28898 27624 VACWR037 KSL 134 29479 29075 VACWR038 K6L 81 29693 29448 VACWR039 K7R 149 + 29832 30281 VACWR088 L1R 250 + 77025 77777 VACWR089 L2R 87 + 77809 78072 VACWR090 L3L 350 79114 78062 VACWR091 L4R 251 + 79139 79894 VACWR092 LSR 128 + 79904 80290 VACWR030 M1L 472 24296 22878 VACWR031 M2L 220 24936 24274 VACWR028 N1L 117 22172 21819 VACWR029 N2L 175 22836 22309 VACWR068 O1L 666 59346 57346 VACWR069 O2L 108 59720 59394
[0444] The foregoing examples are intended only to illustrate certain embodiments of the invention and are not to be construed as limitations. Those variations that would be apparent to one of ordinary skill are also included within the scope of the present invention. One of ordinary skill will recognize that many aspects and embodiments of the invention described herein may be combined, and the invention expressly includes such combinations of the various aspects and embodiments described.