Microarray based multiplex pathogen analysis and uses thereof
11512307 · 2022-11-29
Assignee
Inventors
- Michael Edward Hogan (Stony Brook, NY, US)
- Melissa Rose May (Tucson, AZ, US)
- Frederick Henry Eggers (Sahuarita, AZ, US)
Cpc classification
C12N15/1086
CHEMISTRY; METALLURGY
C12Q2565/513
CHEMISTRY; METALLURGY
G01N33/5308
PHYSICS
C12Q2565/513
CHEMISTRY; METALLURGY
International classification
C40B60/04
CHEMISTRY; METALLURGY
C12N15/10
CHEMISTRY; METALLURGY
Abstract
Provided herein is a 3-dimensional lattice microarray system for DNA sequence detection and analysis. The system has a plurality of bifunctional polymer linkers, on one end of which are attached nucleic acid probes where each have a sequence complementary to signature nucleotide sequences in pathogens, plants or animals. The other end of the bifunctional polymer linker is attached to a solid support by non-covalent or covalent means. Each of the nucleic acid probes have terminal thymidine bases at the 5′ and 3′ ends that permit attachment of the probes to the bifunctional polymer linkers. Also provided is a customizable microarray kit is provided that contains the solid support, linkers, probes, solvent mixture and instructions to use the kit.
Claims
1. A microarray system consisting of: a substantially flat borosilicate glass slide with a front surface consisting of: (1) activated surface moieties selected from the group consisting of an epoxysilane group, an N-hydroxysuccinimide group and an activated carboxylic acid ester attached to the front surface; and (2) a plurality of oligodeoxythymidine linkers each covalently coupled at its 3′ terminus via an amide bond to one of the activated surface moiety groups; wherein there are a greater number of activated surface moieties attached to the front surface of the substantially flat borosilicate glass slide as compared to the total number of covalently coupled oligodeoxythymidine linkers in the plurality thereof, and wherein the activated surface moieties that are not covalently coupled create a lattice width spacing between the covalently coupled plurality of oligodeoxythymidine linkers, each oligodeoxythymidine linker of said plurality of oligodeoxythymidine linkers consisting of: (a) 20 to 60 thymidine bases, with its 5′ terminus covalently linked to a fluorescent label; and (b) a plurality of nucleic acid probes selected from the group consisting of a plurality of pathogenic bacterial nucleotide probes selected from the group consisting of SEQ ID NOS: 37-85, a plurality of pathogenic fungal nucleotide probes selected from the group consisting of SEQ ID NOS: 86-125, and a combination thereof, wherein each of said pathogenic bacterial nucleotide sequences probes of SEQ ID NOS: 37-85 and each of said pathogenic fungal nucleotide sequences probes of SEQ ID NOS: 86-126 consists of a pathogenic bacterial nucleotide sequence or a pathogenic fungal nucleotide sequence sandwiched between two to seven consecutive thymidine nucleotides attached to both the 3′ terminus and to the 5′ terminus of each pathogenic bacterial nucleotide sequence and each pathogenic fungal nucleotide sequence; wherein a thymidine nucleotide at the 3′ terminus and a thymidine nucleotide at the 5′ terminus of each of the plurality of nucleic acid probes is crosslinked to two adjacent oligodeoxythymidine linkers of the plurality of oligodeoxythymidine linkers attached to the substantially flat borosilicate glass slide; and wherein each of the plurality of nucleic acid probes crosslinked at the 3′ terminus and the 5′ terminus to two adjacent oligodeoxythymidine linkers that are covalently coupled to the substantially flat borosilicate glass slide are separated by both a vertical space and the lattice width, such that they form a 3-dimensional lattice on the substantially flat borosilicate glass slide.
Description
BRIEF DESCRIPTION OF THE DRAWINGS
(1) These and other features, aspects, and advantages of the embodiments of the present disclosure will become better understood when the following detailed description is read with reference to the accompanying drawings in which like characters represent like parts throughout the drawing, wherein:
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DETAILED DESCRIPTION OF THE INVENTION
(25) In one embodiment of this invention, there is provided a 3-dimensional lattice microarray system for screening a sample for the presence of a multiplicity of DNA. The system comprises a chemically activatable solid support, a bifunctional polymer linker and a plurality of nucleic acid probes designed to identify sequence determinants in plant, animal or pathogen DNA.
(26) In this embodiment, the solid support may be made of any suitable material known in the art including but not limited to borosilicate glass, a thermoplastic acrylic resin such as poly(methylmethacrylate-VSUVT (PMMA-VSUVT), a cycloolefin polymers such as ZEONOR® 1060R, metals including, but not limited to gold and platinum, plastics including, but not limited to polyethylene terephthalate, polycarbonate, nylon, ceramics including, but not limited to TiO.sub.2, and Indium tin oxide (ITO) and engineered carbon surfaces including, but not limited to graphene. The solid support has a front surface and a back surface and may be activated on the front surface with suitable chemicals which include but are not limited to epoxysilane, isocyanate, succinimide, carbodiimide, aldehyde and maleimide. These are well known in the art and one of ordinary skill in this art would be able to readily functionalize any of these supports as desired. In a preferred embodiment, the solid support is epoxysilane functionalized borosilicate glass support.
(27) In this embodiment, the bifunctional polymer linker has a top domain and a bottom end. On the bottom end is attached a first reactive moiety that allows covalent attachment to the chemically activatable groups in the solid support. Examples of first reactive moieties include but are not limited to an amine group, a thiol group and an aldehyde group. Preferably, the first reactive moiety is an amine group. On the top domain of the bifunctional polymer linker is provided a second reactive moiety that allows covalent attachment to the oligonucleotide probe. Examples of second reactive moieties include but are not limited to nucleotide bases like thymidine, adenine, guanine, cytidine, uracil and bromodeoxyuridine and amino acid like cysteine, phenylalanine, tyrosine glycine, serine, tryptophan, cystine, methionine, histidine, arginine and lysine. The bifunctional polymer linker may be an oligonucleotide such as OligodT, an amino polysaccharide such as chitosan, a polyamine such as spermine, spermidine, cadaverine and putrescine, a polyamino acid, with a lysine or histidine, or any other polymeric compounds with dual functional groups which can be attached to the chemically activatable solid support on the bottom end, and the nucleic acid probes on the top domain. Preferably, the bifunctional polymer linker is OligodT having an amine group at the 5′ end.
(28) In this embodiment, the bifunctional polymer linker may be unmodified. Alternatively, the bifunctional polymer linker has a color or fluorescent label attached covalently. Examples of fluorescent labels include, but are not limited to a Cy5, a DYLIGHT™ DY647, a ALEXA FLUOR® 647, a Cy3, a DYLIGHT™ DY547, or a ALEXA FLUOR® 550. These may be attached to any reactive group including but not limited to, amine, thiol, aldehyde, sugar amido and carboxy on the bifunctional polymer linker. The chemistries of such reactive groups are well known in the art and one or ordinary skill can readily identify a suitable group on a selected bifunctional polymer linker for attaching the fluorescent label. Preferably, the bifunctional polymer linker is Cy5-labeled OligodT having an amino group attached at its 3′terminus for covalent attachment to an activated surface on the solid support.
(29) Also in this embodiment, the present invention provides a plurality of nucleic acid probes designed with the purpose of identifying sequence determinants in plants, animals or pathogens. The nucleic acid probes are synthetic oligonucleotides and have terminal thymidine bases at their 5′ and 3′ end. The thymidine bases permit covalent attachment of the nucleic acid probes to the bifunctional polymer linker by any standard coupling procedures including but not limited to chemical, photochemical and thermal coupling. Preferably, covalent attachment of the nucleic acid probes to the bifunctional polymer linker is by photochemical means using ultraviolet light.
(30) In this embodiment, the fluorescent label (fluorescent tag) attached to the bifunctional polymer linker is beneficial since it allows the user to image and detect the position of the individual nucleic acid probes (“spot”) printed on the microarray. By using two different fluorescent labels, one for the bifunctional polymer linker and the second for the amplicons generated from the DNA being queried, the user can obtain a superimposed image that allows parallel detection of those nucleic acid probes which have been hybridized with amplicons. This is advantageous since it helps in identifying the plant or pathogen comprised in the sample using suitable computer and software, assisted by a database correlating nucleic acid probe sequence and microarray location of this sequence with a known DNA signature in plants, animals or pathogens. Any emitter/acceptor fluorescent label pairs known in the art may be used. For example, the bifunctional polymer linker may be labeled with emitters such as a Cy5, DYLIGHT™ DY647, or ALEXA FLUOR® 647, while the amplicons may be labeled with acceptors such as Cy3, DYLIGHT™ DY547, or ALEXA FLUOR® 550. Preferably, the emitter is Cy5 and the acceptor is Cy3.
(31) In another embodiment of this invention, there is provided a 3-dimensional lattice microarray system for screening a sample for the presence of a multiplicity of DNA. The system comprises a solid support, a fluorescent labeled bifunctional polymer linker and a plurality of nucleic acid probes designed to identify sequence determinants in plant, animal or pathogen DNA.
(32) In this embodiment, the solid support has a front surface and a back surface. The front surface has non-covalent adsorptive properties for specific functionalized group(s) present in the fluorescent labeled bifunctional polymer linker (described below). Examples of such solid support include, but are not limited to borosilicate glass, SiO2, metals including, but not limited to gold and platinum, plastics including, but not limited to polyethylene terephthalate, polycarbonate, nylon, ceramics including, but not limited to TiO.sub.2, and Indium tin oxide (ITO) and engineered carbon surfaces including, but not limited to graphene.
(33) In this embodiment, the fluorescent labeled bifunctional polymer linker has a top domain and a bottom end. On the bottom end is attached one or more functional groups (designated by “R.sub.n”) that are compatible for non-covalent adsorptive attachment with the front surface of the solid support. Examples of compatible R groups include, but are not limited to, single stranded nucleic acids (example, OligodT), amine-polysaccharide (example, chitosan), extended planar hydrophobic groups (example, digoxigenin, pyrene, Cy-5 dye).
(34) Further in this embodiment, on the top domain of the bifunctional polymer linker is provided a second reactive moiety that allows covalent attachment to the oligonucleotide probe. Examples of second reactive moieties include but are not limited to nucleotide bases like thymidine, adenine, guanine, cytidine, uracil and bromodeoxyuridine and amino acid like cysteine, phenylalanine, tyrosine glycine, serine, tryptophan, cystine, methionine, histidine, arginine and lysine. To the bottom end of the bifunctional polymer linker may be attached polymeric molecules including, but not limited to an oligonucleotide such as OligodT, an amino polysaccharide such as chitosan, a polyamine such as spermine, spermidine, cadaverine and putrescine, a polyamino acid, with a lysine or histidine, or OligodT that is modified at its 5′ end with a digoxigenin, a pyrene or a Cy5 or any other polymeric molecules with or without chemical modification suitable for non-covalent attachment to the solid support. On the top domain of these bifunctional polymer linkers is attached, the nucleic acid probes. Preferably, the bifunctional polymer linker is OligodT.
(35) In one aspect of this embodiment, the bifunctional polymer linker is unmodified. Alternatively, the bifunctional polymer linker may be a fluorescent labeled bifunctional polymer linker. The fluorescent label may be, but is not limited to a Cy5, a DYLIGHT™ DY647, a ALEXA FLUOR® 647, a Cy3, a DYLIGHT™ DY547, or a ALEXA FLUOR® 550 attached to any reactive group including but not limited to, amine, thiol, aldehyde, sugar amido and carboxy on the bifunctional polymer linker. The chemistries of such reactive groups are well known in the art and one or ordinary skill can readily identify a suitable group on a selected bifunctional polymer linker for attaching the fluorescent label. Preferably, the bifunctional polymer linker is Cy5-labeled OligodT.
(36) Also in this embodiment, the present invention provides a plurality of nucleic acid probes designed with the purpose of identifying sequence determinants in plants, animals or pathogens. The nucleic acid probes are synthetic oligonucleotides and have terminal thymidine bases at their 5′ and 3′ end. The thymidine bases permit covalent attachment of the nucleic acid probes to the bifunctional polymer linker by any standard coupling procedures including but not limited to chemical, photochemical and thermal coupling. Preferably, covalent attachment of the nucleic acid probes to the bifunctional polymer linker is by photochemical means using ultraviolet light.
(37) In this embodiment, the fluorescent label (fluorescent tag) attached to the bifunctional polymer linker is beneficial since it allows the user to image and detect the position of the individual nucleic acid probes (“spot”) printed on the microarray. By using two different fluorescent labels, one for the bifunctional polymer linker and the second for the amplicons generated from the DNA being queried, the user can obtain a superimposed image that allows parallel detection of those nucleic acid probes which have been hybridized with amplicons. This is advantageous since it helps in identifying the plant or pathogen comprised in the sample using suitable computer and software, assisted by a database correlating nucleic acid probe sequence and microarray location of this sequence with a known DNA signature in plants, animals or pathogens. Any emitter/acceptor fluorescent label pairs known in the art may be used. For example, the bifunctional polymer linker may be labeled with emitters such as a Cy5, DYLIGHT™ DY647, or ALEXA FLUOR® 647, while the amplicons may be labeled with acceptors such as Cy3, DYLIGHT™ DY547, or ALEXA FLUOR® 550. Preferably, the emitter is Cy5 and the acceptor is Cy3.
(38) In yet another embodiment of this invention, there is provided a method for fabricating a 3-dimensional lattice microarray system for the purpose of screening a sample for the presence of a multiplicity of DNA in a sample. The method comprises, contacting a solid support with a formulation comprising a plurality of nucleic acid probes, a plurality of fluorescent bifunctional polymer linkers and a solvent mixture comprising water and a high boiling point, water-miscible liquid, allowing a first attachment between the fluorescent bifunctional polymer linkers and the solid support to proceed, evaporating the water in the solvent mixture thereby concentrating the nucleic acid probes and fluorescent labeled bifunctional polymer linkers, allowing a second attachment between the nucleic acid probes and the fluorescent bifunctional polymer linker, and washing the solid support with at least once to remove unattached fluorescent bifunctional polymer linkers and nucleic acid probes.
(39) In this embodiment, the contacting step is achieved by standard printing methods known in the art including, but not limited to piezo-electric printing, contact printing, ink jet printing and pipetting, which allow an uniform application of the formulation on the activated support. For this, any suitable solid support known in the art including but not limited to borosilicate glass, a polycarbonate, a graphene, a gold, a thermoplastic acrylic resin such as poly(methylmethacrylate-VSUVT (PMMA-VSUVT) and a cycloolefin polymer such as ZEONOR® 1060R may be employed.
(40) In one aspect of this embodiment, the first attachment of the bifunctional polymer linker to the solid support is by non-covalent means such as by adsorption or electrostatic binding. In this case, the bifunctional polymer linkers with one or more functional groups (designated by “R.sub.n”) on the bottom end, that are compatible for attachment with the front surface of the solid support will be used. Examples of compatible R groups include, but are not limited to, single stranded nucleic acids (example, OligodT), amine-polysaccharide (example, chitosan), extended planar hydrophobic groups (example, digoxigenin, pyrene, Cy-5 dye). In another aspect of this embodiment, the first attachment of the bifunctional polymer linker to the solid support is by covalent coupling between chemically activatable groups on the solid support and a first reactive moiety on the bottom end of the bifunctional polymer linker. Suitable chemicals including but are not limited to epoxysilane, isocyanate, succinimide, carbodiimide, aldehyde and maleimide may be used for activating the support. These are well known in the art and one of ordinary skill in this art would be able to readily functionalize any of these supports as desired. In a preferred embodiment, a borosilicate glass support that is epoxysilane functionalized is used. Examples of first reactive moieties amenable to covalent first attachment include, but are not limited to an amine group, a thiol group and an aldehyde group. Preferably, the first reactive moiety is an amine group.
(41) In this embodiment, the bifunctional polymer linker has a second reactive moiety attached at the top domain. Examples of second reactive moieties include but are not limited to nucleotide bases like thymidine, adenine, guanine, cytidine, uracil and bromodeoxyuridine and amino acid like cysteine, phenylalanine, tyrosine glycine, serine, tryptophan, cystine, methionine, histidine, arginine and lysine. Preferably, the second reactive moiety is thymidine. In this aspect of the invention, the bifunctional polymer linker may be an oligonucleotide such as OligodT, an amino polysaccharide such as chitosan, a polyamine such as spermine, spermidine, cadaverine and putrescine, a polyamino acid, with a lysine or histidine, or any other polymeric compounds with dual functional groups which can be attached to the chemically activatable solid support on the bottom end, and the nucleic acid probes on the top domain. Preferably, the bifunctional polymer linker is OligodT having an amine group at the 5′ end.
(42) In this embodiment, the bifunctional polymer linkers are modified with a fluorescent label. Examples of fluorescent labels include but are not limited Cy5, DYLIGHT™ DY647, ALEXA FLUOR® 647, Cy3, DYLIGHT™ DY547 and ALEXA FLUOR® 550 attached to any reactive group including but not limited to, amine, thiol, aldehyde, sugar amido and carboxy on the bifunctional polymer linker. The chemistries of such reactive groups are well known in the art and one or ordinary skill can readily identify a suitable group on a selected bifunctional polymer linker for attaching the fluorescent label. Preferably, the bifunctional polymer linker used for fabricating the microarray is Cy5-labeled OligodT.
(43) The method of fabricating the microarray requires use of a solvent mixture comprising water and a water-miscible liquid having a boiling point above 100° C. This liquid may be any suitable water-miscible liquid with a boiling point higher than that of water, so that all the solvent is not lost during the evaporation step. This allows the molecular reactants—nucleic acid probes and bifunctional linkers to be progressively concentrated during evaporation. Such controlled evaporation is crucial to the present invention since it controls the vertical spacing between nucleic acid probes their avoiding steric hindrance during the hybridization steps thereby improving accuracy and precision of the microarray. Examples of high boiling point water-miscible solvent include but are not limited to glycerol, DMSO and propanediol. The ratio or water to high boiling point solvent is kept between 10:1 and 100:1 whereby, in the two extremes, upon equilibrium, volume of the fluid phase will reduce due to water evaporation to between 1/100th and 1/10.sup.th of the original volume, thus giving rise to a 100-fold to 10-fold increase in reactant concentration. In a preferred embodiment, the water-miscible solvent is propanediol and the water to propanediol ratio is 100:1.
(44) Further in this embodiment, the nucleic acid probes used in the method of microarray fabrication are designed with terminal thymidine bases at their 5′ and 3′ end. The thymidine bases permit covalent attachment of the nucleic acid probes to the bifunctional polymer linker by any standard coupling procedures including but not limited to chemical, photochemical and thermal coupling during the fabrication process. Preferably, coupling of the nucleic acid probes to the fluorescent labeled bifunctional polymer linkers is by photochemical covalent crosslinking.
(45) In yet another embodiment of this invention, there is provided a customizable microarray kit. The kit comprises a solid support, a plurality of fluorescent labeled bifunctional polymer linkers, nucleic acid probes and a solvent mixture comprising water and one or more of a water-miscible liquid having a boiling point above 100° C., and instructions to use the kit. Each of the components comprising this kit may be individually customized prior to shipping based on the goals of the end user.
(46) In this embodiment, the solid support has a front surface and a back surface and made of any suitable material known in the art including but not limited to borosilicate glass, a polycarbonate, a graphene, a gold, a thermoplastic acrylic resin such as poly(methylmethacrylate-VSUVT (PMMA-VSUVT) and a cycloolefin polymer such as sold under the trademark ZEON® 1060R owned by Zeon Chemicals.
(47) In one aspect of this embodiment, the solid support is unmodified and has properties capable of non-covalent attachment to groups in the bifunctional polymer linker. Alternatively, the solid support is activated on the front surface with chemically activatable groups which include but are not limited to epoxysilane, isocyanate, succinimide, carbodiimide, aldehyde and maleimide. These are well known in the art and one of ordinary skill in this art would be able to readily functionalize any of these supports as desired. In a preferred embodiment, the solid support is epoxysilane functionalized borosilicate glass support.
(48) In this embodiment, the bifunctional polymer linker has a top domain and a bottom end. In one aspect of this embodiment, to the bottom end of the bifunctional polymer linker are attached one or more functional groups (designated by “R.sub.n”), which are compatible for attachment with the front surface of the solid support in a non-covalent binding. Examples of such compatible R groups include, but are not limited to, single stranded nucleic acids (example, OligodT), amine-polysaccharide (example, chitosan), extended planar hydrophobic groups (example, digoxigenin, pyrene, Cy-5 dye). Alternatively, to the bottom end of the bifunctional polymer linker are attached a first reactive moiety that allows covalent attachment to chemically activatable groups in the solid support. Examples of first reactive moieties include but are not limited to an amine group, a thiol group and an aldehyde group. Preferably, the first reactive moiety is an amine group.
(49) Further in this embodiment, on the top domain of the bifunctional polymer linker is provided a second reactive moiety that allows covalent attachment to the oligonucleotide probe. Examples of second reactive moieties include but are not limited to nucleotide bases like thymidine, adenine, guanine, cytidine, uracil and bromodeoxyuridine and amino acid like cysteine, phenylalanine, tyrosine glycine, serine, tryptophan, cystine, methionine, histidine, arginine and lysine. The bifunctional polymer linker may be an oligonucleotide such as OligodT, an amino polysaccharide such as chitosan, a polyamine such as spermine, spermidine, cadaverine and putrescine, a polyamino acid, with a lysine or histidine, or any other polymeric compounds with dual functional groups for attachment to the solid support from the bottom end, and the nucleic acid probes from the top domain.
(50) In one aspect of this embodiment, the bifunctional polymer linkers are modified with a fluorescent label. Alternatively, the bifunctional polymer linker may be a fluorescent labeled bifunctional polymer linker where the fluorescent label is a fluorescent cyanine dye Cy5 or Cy3, a fluorescent phosphoramidite dye sold under the trademark DYLIGHT™ DY647 or DYLIGHT™ DY547, or a fluorescent dye sold under the trademark ALEXA FLUOR® 647 all owned by Thermo Fisher Scientific Inc attached to any reactive group including but not limited to, amine, thiol, aldehyde, sugar amido and carboxy on the bifunctional polymer linker. The chemistries of such reactive groups are well known in the art and one or ordinary skill can readily identify a suitable group on a selected bifunctional polymer linker for attaching the fluorescent label. Preferably, the bifunctional polymer linker is Cy5-labeled OligodT.
(51) Also in this embodiment, the present invention provides a plurality of nucleic acid probes designed with the purpose of identifying sequence determinants in plants, animals or pathogens. The nucleic acid probes are synthetic oligonucleotides and have terminal thymidine bases at their 5′ and 3′ end. The thymidine bases permit covalent attachment of the nucleic acid probes to the bifunctional polymer linker by any standard coupling procedures including but not limited to chemical, photochemical and thermal coupling. Preferably, covalent attachment of the nucleic acid probes to the bifunctional polymer linker is by photochemical means using ultraviolet light.
(52) In yet another embodiment of this invention there is provided a method for detecting the presence of one or more pathogens in a plant sample. In this embodiment, the pathogen may be a human pathogen, an animal pathogen or a plant pathogen, such as a bacterium, a fungus, a virus, a yeast, algae or a protozoan or a combination thereof. These pathogens may be present as constituents of the soil, soilless growth media, hydroponic growth media or water in which the plant sample was grown. The method comprises harvesting the pathogens from the plant sample, isolating total nucleic acids comprising pathogen DNA, performing a first amplification for generating one or more amplicons from the one or more pathogens present in the sample in a single, simultaneous step; performing a labeling amplification using as template, the one or more amplicons generated in the first amplification step to generate fluorescent labeled second amplicons; hybridizing the second amplicons with the nucleic acid probes immobilized on the fabricated self-assembled, 3-dimensional lattice microarray described above and imaging the microarray to detect the fluorescent signal, which indicates presence of the one or more pathogens in a plant sample. In this embodiment, the pathogens present on the plant surface may be harvested by washing the plant with water to recover the pathogens, followed by concentrating by filtration on a sterile 0.4 μm filter. In another aspect of this embodiment, pathogens within the plant tissue may be harvested by fluidizing the plant tissue sample and pathogens, followed by centrifuging to get a pellet of plant cells and pathogen cells. In either embodiment, the harvested sample is disrupted to release the total nucleic acids which is used in the subsequent steps without further purification.
(53) Also in this embodiment, the sample comprising nucleic acids from pathogens (external pathogens) or nucleic acids from both pathogens and plant (internal pathogens) is used to perform a first amplification of pathogen DNA using pathogen-specific first primer pairs to obtain one or more pathogen-specific first amplicons. Any DNA amplification methodology, including loop-mediated isothermal amplification (LAMP) or polymerase chain reaction (PCR) that can selectively amplify the DNA complement in the sample may be employed. In a preferred embodiment, the amplification is by PCR. In one embodiment, the pathogen is a bacterium and the first primer pairs have sequences shown in SEQ ID NOS: 1-12. In another embodiment, the pathogen is a fungus and the first primer pairs have sequences shown in SEQ ID NOS: 13-16. An aliquot of first amplicons so generated is used as template for a second, labelling PCR amplification using fluorescent labeled second primer pairs. The second primer pairs are designed to amplify an internal flanking region in the one or more first amplicons to obtain one or more first fluorescent labeled second amplicons. In one embodiment, the pathogen is a bacterium and the second primer pairs have sequences shown in SEQ ID NOS: 19-30. In another embodiment, the pathogen is a fungus and the second primer pairs have sequences shown in SEQ ID NOS: 31-34.
(54) Further in this embodiment, the fluorescent labeled second amplicons are hybridized on a 3-dimensional lattice microarray system having a plurality of nucleic acid probes as described in detail above. In this embodiment, the bifunctional polymer linker has a fluorescent label (that is different from the label on the second amplicon) attached whereby, imaging the microarray after hybridization and washing results in two distinct fluorescent signals—the signal from the fluorescent bifunctional polymer linker which is covalently linked to the nucleic acid probe during fabrication, which would be detected in each spot comprised in the microarray, and a second amplicon signal that would be detected only in those spots where the nucleic acid probe sequence is complementary to the second amplicon (originally derived by amplification from the pathogen DNA in the sample). Thus, superimposing the two images using a computer provides beneficial attributes to the system and method claimed in this invention since one can readily identify the plant or pathogen comprised in the sample from a database that correlates nucleic acid probe sequence and microarray location of this sequence with a known DNA signature in plants or pathogens. In a preferred embodiment, the bacterial nucleic acid probes having sequences shown in SEQ ID NOS: 37-85. and fungal nucleic acid probes having sequences shown in SEQ ID NOS: 86-125 may be used for this purpose.
(55) Further to this embodiment is a method for detecting plant DNA. The plant may be a terrestrial plant such as a Humulus or a Cannabis, an aquatic plant, an epiphytic plant or a lithophytic plant that grows in soil, soilless media, hydroponic growth media or water. In a preferred aspect, the plant is a Cannabis. This method comprises the steps of performing an amplification on an unpurified complex nucleic acid sample using plant-specific first primer pairs to generate plant-specific first amplicons. In one aspect of this embodiment, the first primer pair has sequences shown in SEQ ID NOS: 17-18. Any DNA amplification methodology, including loop-mediated isothermal amplification (LAMP) or polymerase chain reaction (PCR) that can selectively amplify the DNA complement in the sample may be employed. Preferably the amplification is by PCR. The first amplicons so generated are used as template for a labeling amplification step using fluorescent labeled second primer pairs that are designed to amplify an internal flanking region in the one or more of first amplicons generated in the first amplification step to generate one or more first fluorescent labeled second amplicons. In one embodiment, the second primer pair has sequences shown in SEQ ID NOS: 35-36. The second amplicons are hybridized on a 3-dimensional lattice microarray system having a plurality of plant-specific nucleic acid probes, and the microarrays imaged and analyzed as described above for identifying pathogen DNA. In one aspect of this embodiment, the hybridization nucleic acid probes have sequences shown in SEQ ID NOS: 126-128.
(56) In yet another embodiment of this invention, there is provided a method for simultaneously detecting resident pathogen DNA and plant DNA in a plant sample in a single assay. In this embodiment, the pathogen may be a human pathogen, an animal pathogen or a plant pathogen, which may be a bacterium, a fungus, a virus, a yeast, algae or a protozoan or a combination thereof. These pathogens may be present as constituents of the soil, soilless growth media, hydroponic growth media or water in which the plant sample was grown. The plant may be a terrestrial plant such as a Humulus or a Cannabis, an aquatic plant, an epiphytic plant or a lithophytic plant that grows in soil, soilless media, hydroponic growth media or water. Preferably, the plant is a Cannabis.
(57) In this embodiment, the method comprises harvesting a plant tissue sample potentially comprising one or more pathogens, fluidizing the plant tissue sample and the one or more pathogens and isolating total nucleic acids comprising DNA from at least the plant tissue and DNA from the one or more pathogens. In one aspect of this embodiment, the step of isolating total nucleic acids comprises centrifuging the fluidized sample to get a pellet of plant cells and pathogen cells which are disrupted to release the total nucleic acids, which are used in the subsequent steps without further purification.
(58) Further in this embodiment, a first amplification is performed on the unpurified total nucleic acid sample using one or more of a first primer pair each selective for the one or more pathogen DNA and one or more of a second primer pair selective for the plant DNA to generate one or more pathogen-specific first amplicons and one or more plant-specific second amplicons. Any DNA amplification methodology, including loop-mediated isothermal amplification (LAMP) or polymerase chain reaction (PCR) that can selectively amplify the DNA complement in the sample may be employed. In a preferred embodiment, the amplification is by PCR. In one embodiment, the pathogen is a bacterium and the first primer pairs have sequences shown in SEQ ID NOS: 1-12. In another embodiment, the pathogen is a fungus and the first primer pairs have sequences shown in SEQ ID NOS: 13-16. In either of these embodiments, the plant-specific second primer pairs have sequences shown in SEQ ID NOS: 35-36. An aliquot of the first and second amplicons so generated is used as a template for a second, labeling PCR amplification step using fluorescent labeled third primer pairs having a sequence complementary to an internal flanking region in the one or more pathogen-specific first amplicons and fluorescent labeled fourth primer pairs having a sequence complementary to an internal flanking region in the one or more plant-specific second amplicons. Any DNA amplification methodology, including loop-mediated isothermal amplification (LAMP) or polymerase chain reaction (PCR) that can selectively amplify the DNA complement in the sample may be employed. In a preferred embodiment, the amplification is by PCR. In one embodiment, the pathogen is a bacterium and the third primer pairs have sequences shown in SEQ ID NOS: 19-30. In another embodiment, the pathogen is a fungus and the third primer pairs have sequences shown in SEQ ID NOS: 31-34. In either of these embodiments, the plant-specific fourth primer pairs have sequences shown in SEQ ID NOS: 35-36. The labeling PCR step results in generation of first fluorescent labeled third amplicons and second fluorescent labeled fourth amplicons corresponding to the pathogen and plant DNA respectively in the original harvested sample. These amplicons are then hybridized on a 3-dimensional lattice microarray system having a plurality of nucleic acid probes specific to sequence determinants in pathogen DNA or plant DNA. Bacterial nucleic acid probes having sequences shown in SEQ ID NOS: 37-85, fungal nucleic acid probes having sequences shown in SEQ ID NOS: 86-125 and plant nucleic acid probes having sequences shown in SEQ ID NOS: 126-128. may be used for this purpose. After hybridization, unhybridized amplicons are removed by washing and the microarray imaged. Detection of the first fluorescent labeled third amplicon signal indicates presence of pathogens in the plant sample. Detecting the second fluorescent labeled fourth amplicon indicates presence of the plant DNA. Superimposing these two signals with the third fluorescent signal from the fluorescent bifunctional polymer linker-coupled nucleic acid probes allow simultaneous identification of the pathogen and plant in the sample by correlating nucleic acid probe sequence and microarray location of this sequence with a known DNA signature in plants or pathogens. These features provide beneficial attributes to the system and method claimed in this invention.
(59) In yet another embodiment of the present disclosure there is provided an improved method for DNA based pathogen analysis. The embodiments of the present disclosure use DNA amplification methodologies, including loop-mediated isothermal amplification (LAMP) or polymerase chain reaction (PCR) tests that can selectively amplify the DNA complement of that plant material using unpurified plant and pathogen material. The embodiments are also based on the use of aforementioned PCR-amplified DNA as the substrate for microarray-based hybridization analysis, wherein the hybridization is made simple because the nucleic acid probes used to interrogate the DNA of such pathogens are optimized to function at room temperature. This enables the use of the above-mentioned microarray test at ambient temperature, thus bypassing the prior art requirement that testing be supported by an exogenous temperature-regulating device.
(60) The following examples are given for the purpose of illustrating various embodiments of the invention and are not meant to limit the present invention in any fashion. One skilled in the art will appreciate readily that the present invention is well adapted to carry out the objects and obtain the ends and advantages mentioned, as well as those objects, ends and advantages inherent herein. Changes therein and other uses which are encompassed within the spirit of the invention as defined by the scope of the claims will occur to those skilled in the art.
Example 1
(61) Fabrication of 3-Dimensional Lattice Microarray Systems
(62) The present invention teaches a way to link a nucleic acid probe to a solid support surface via the use of a bifunctional polymeric linker. The nucleic acid probe can be a PCR amplicon, synthetic oligonucleotides, isothermal amplification products, plasmids or genomic DNA fragment in a single stranded or double stranded form. The invention can be sub-divided into two classes, based on the nature of the underlying surface to which the nucleic acid probe would be linked.
(63) 1. Covalent Microarray System with Activated Solid Support.
(64) The covalent attachment of any one of these nucleic acid probes does not occur to the underlying surface directly, but is instead mediated through a relatively long, bi-functional polymeric linker that is capable of both chemical reaction with the surface and also capable of efficient UV-initiated crosslinking with the nucleic acid probe. The mechanics of this process is spontaneous 3D self assembly and is illustrated in
(65) (a) an unmodified nucleic acid probe 3 such as an oligonucleotide, PCR or isothermal amplicon, plasmid or genomic DNA;
(66) (b) a chemically activatable surface 1 with chemically activatable groups (designated “X”) compatible for reacting with a primary amine such as. epoxysilane, isocyanate, succinimide, carbodiimide, aldehyde.
(67) (c) bifunctional polymer linkers 2 such as a natural or modified OligodT, amino polysaccharide, amino polypeptide suitable for coupling to chemically activatable groups on the support surface, each attached with a fluorescent label 4; and
(68) (d) a solvent comprising water and a high boiling point, water-miscible liquid such as glycerol, DMSO or propanediol (water to solvent ratio between 10:1 and 100:1).
(69) Table 1 shows examples of chemically activatable groups and matched reactive groups on the bifunctional polymer linker for mere illustration purposes only and does not in any way preclude use of other combinations of matched reactive pairs.
(70) TABLE-US-00001 TABLE 1 Covalent Attachment of Bifunctional Polymeric Linker to an Activated Surfaces Activated Surface Matched Reactive Group Specific Implementation as Bifunctional Moiety on Bifunctional Linker polymeric linker Epoxysilane Primary Amine (1) Amine-modified OligodT (20-60 bases) (2) Chitosan (20-60 subunits) (3) Lysine containing polypeptide (20-60aa) EDC Activated Primary Amine (4) Amine-modified OligodT (20-60 bases) Carboxylic Acid (5) Chitosan (20-60 subunits) (6) Lysine containing polypeptide (20-60aa) N-hydroxysuccinimide Primary Amine (7) Amine-modified OligodT (20-60 bases) (NHS) (8) Chitosan (20-60 subunits) (9) Lysine containing polypeptide (20-60aa)
(71) When used in the present invention, the chemically activatable surface, bifunctional polymer linkers and unmodified nucleic acid probes are included as a solution to be applied to a chemically activated surface 4 by ordinary methods of fabrication used to generate DNA Hybridization tests such as contact printing, piezo electric printing, ink jet printing, or pipetting.
(72) Microarray fabrication begins with application of a mixture of the chemically activatable surface, bifunctional polymer linkers and unmodified nucleic acid probes to the surface. The first step is reaction and covalent attachment of the bifunctional linker to the activated surface (
(73) In the second step, the water in the solvent is evaporated to concentrate the DNA and bifunctional linker via evaporation of water from the solvent (
(74) In the third step, the terminal Thymidine bases in the nucleic acid probes are UV crosslinked to the bifunctional linker within the evaporated surface (
(75) 2. Microarray System with Unmodified Solid Support for Non-Covalent Attachment
(76) In this microarray system, attachment of the nucleic acid probes does not occur to the underlying surface directly, but is instead mediated through a relatively long, bi-functional polymeric linker that binds non-covalently with the solid support, but covalently with the nucleic acid probes via UV-initiated crosslinking. The mechanics of this process is spontaneous 3D self assembly and is illustrated in
(77) Table 2 shows examples of unmodified support surfaces and matched absorptive groups on the bifunctional polymer linker for mere illustration purposes only and does not in any way precludes the use of other combinations of these.
(78) TABLE-US-00002 TABLE 2 Non-Covalent Attachment of Bi-Functional Polymeric Linker to an Inert Surface Representative Matched Adsorptive Group Specific Bifunctional support surface on Bifunctional Linker (R.sub.n) polymeric linker glass Single Stranded Nucleic OligodT (30-60 bases) Acid > 10 bases glass Amine-Polysaccharide Chitosan (30-60 subunits) glass Extended Planar Hydrophobic OligodT (30-60 bases)- Groups e.g. Digoxigenin 5′-Digoxigenin polycarbonate Single Stranded Nucleic Oligo-dT (30-60 bases) Acid > 10 bases polycarbonate Amine-Polysaccharide Chitosan (30-60 subunits) polycarbonate Extended Planar Hydrophobic OligodT (30-60 bases)- Groups e.g. Digoxigenin 5′-Digoxigenin graphene Extended Planar Hydrophobic OligodT (30-60 bases)- Groups e.g. pyrene 5′pyrene graphene Extended Planar Hydrophobic OligodT (30-60 bases)- Groups e.g. CY-5 dye 5′-CY-5 dye graphene Extended Planar Hydrophobic OligodT (30-60 bases)- Groups e.g. Digoxigenin 5′-Digoxigenin gold Extended Planar Hydrophobic OligodT (30-60 bases)- Groups e.g. pyrene 5′pyrene gold Extended Planar Hydrophobic OligodT (30-60 bases)- Groups e.g. CY-5 dye 5′ CY-5 dye gold Extended Planar Hydrophobic OligodT (30-60 bases)- Groups e.g. Digoxigenin 5′ Digoxigenin
(79) When used in the present invention, components 1-3 are included as a solution to be applied to the solid support surface by ordinary methods of fabrication used to generate DNA Hybridization tests such as contact printing, piezo electric printing, ink jet printing, or pipetting.
(80) Microarray fabrication begins with application of a mixture of the components (1)-(3) to the surface. The first step is adsorption of the bifunctional linker to the support surface (
(81) In the second step, the water in the solvent is evaporated to concentrate the DNA and bifunctional linker via evaporation of water from the solvent (
(82) In the third step, the terminal Thymidine bases in the nucleic acid probes are UV crosslinked to the bifunctional linker within the evaporated surface (
(83) Although such non-covalent adsorption described in the first step is generally weak and reversible, when occurring in isolation, in the present invention it is taught that if many such weak adsorptive events between the bifunctional polymeric linker and the underlying surface occur in close proximity, and if the closely packed polymeric linkers are subsequently linked to each other via Thymidine-mediated photochemical crosslinking, the newly created extended, multi-molecular (crosslinked) complex will be additionally stabilized on the surface, thus creating a stable complex with the surface in the absence of direct covalent bonding to that surface.
(84) The present invention works very efficiently for the linkage of synthetic oligonucleotides as nucleic acid probes to form a microarray-based hybridization device for the analysis of microbial DNA targets. However, it is clear that the same invention may be used to link PCR amplicons, synthetic oligonucleotides, isothermal amplification products, plasmid DNA or genomic DNA fragment as nucleic acid probes. It is also clear that the same technology could be used to manufacture hybridization devices that are not microarrays.
(85) DNA nucleic acid probes were formulated as described in Table 3, to be deployed as described above and illustrated in
(86) TABLE-US-00003 TABLE 3 Representative Conditions of use of the Present Invention 5′ labelled Unique sequence OligodT Oligonucleotide Fluorescent Nucleic acid probe 30-38 bases Long marker 30 bases Type 7 T's at each end Long(marker) Nucleic acid probe 50 mM 0.15 mM Concentration Bifunctional Linker OligodT 30 bases long Primary amine at 3′ terminus Bifunctional Linker 1 mM Concentration High Boiling point Water: Propanediol, Solvent 100:1 Surface Epoxysilane on borosilicate glass UV Crosslinking Dose 300 millijoule (mjoule)
(87) TABLE-US-00004 TABLE 4 Nucleic acid probes Linked to the Microarray Surface via the Present Invention SEQ ID NO: 132 Negative control TTTTTTCTACTACCTATGCTGATTCACTCTTTTT SEQ ID NO: 129 Imager Calibration TTTTCTATGTATCGATGTTGAGAAATTTTTTT (High) SEQ ID NO: 130 Imager Calibration (Low) TTTTCTAGATACTTGTGTAAGTGAATTTTTTT SEQ ID NO: 131 Imager Calibration TTTTCTAAGTCATGTTGTTGAAGAATTTTTTT (Medium) SEQ ID NO: 126 Cannabis ITS1 DNA TTTTTTAATCTGCGCCAAGGAACAATATTTTTTT Control 1 SEQ ID NO: 127 Cannabis ITS1 DNA TTTTTGCAATCTGCGCCAAGGAACAATATTTTTT Control 2 SEQ ID NO: 128 Cannabis ITS1 DNA TTTATTTCTTGCGCCAAGGAACAATATTTTATTT Control 3 SEQ ID NO: 86 Total Yeast and Mold TTTTTTTTGAATCATCGARTCTTTGAACGCATTTTTTT (High sensitivity) SEQ ID NO: 87 Total Yeast and Mold TTTTTTTTGAATCATCGARTCTCCTTTTTTT (Low sensitivity) SEQ ID NO: 88 Total Yeast and Mold TTTTTTTTGAATCATCGARTCTTTGAACGTTTTTTT (Medium sensitivity) SEQ ID NO: 132 Negative control TTTTTTCTACTACCTATGCTGATTCACTCTTTTT SEQ ID NO: 92 Aspergillus fumigatus 1 TTTCTTTTCGACACCCAACTTTATTTCCTTATTT SEQ ID NO: 90 Aspergillus flavus 1 TTTTTTCGCAAATCAATCTTTTTCCAGTCTTTTT SEQ ID NO: 95 Aspergillus niger 1 TTTTTTCGACGTTTTCCAACCATTTCTTTT SEQ ID NO: 100 Botrytis spp. TTTTTTTCATCTCTCGTTACAGGTTCTCGGTTCTTTTTTT SEQ ID NO: 108 Fusarium spp. TTTTTTTTAACACCTCGCRACTGGAGATTTTTTT SEQ ID NO: 89 Alternaria spp TTTTTTCAAAGGTCTAGCATCCATTAAGTTTTTT SEQ ID NO: 123 Rhodoturula spp. TTTTTTCTCGTTCGTAATGCATTAGCACTTTTTT SEQ ID NO: 117 Penicillium paxilli TTTTTTCCCCTCAATCTTTAACCAGGCCTTTTTT SEQ ID NO: 116 Penicillium oxalicum TTTTTTACACCATCAATCTTAACCAGGCCTTTTT SEQ ID NO: 118 Penicillium spp. TTTTTTCAACCCAAATTTTTATCCAGGCCTTTTT SEQ ID NO: 102 Candida spp. Group 1 TTTTTTTGTTTGGTGTTGAGCRATACGTATTTTT SEQ ID NO: 103 Candida spp. Group 2 TTTTACTGTTTGGTAATGAGTGATACTCTCATTTT SEQ ID NO: 124 Stachybotrys spp TTTCTTCTGCATCGGAGCTCAGCGCGTTTTATTT SEQ ID NO: 125 Trichoderma spp. TTTTTCCTCCTGCGCAGTAGTTTGCACATCTTTT SEQ ID NO: 105 Cladosporium spp. TTTTTTTTGTGGAAACTATTCGCTAAAGTTTTTT SEQ ID NO: 121 Podosphaera spp. TTTTTTTTAGTCAYGTATCTCGCGACAGTTTTTT SEQ ID NO: 132 Negative control TTTTTTCTACTACCTATGCTGATTCACTCTTTTT SEQ ID NO: 37 Total Aerobic bacteria TTTTTTTTTCCTACGGGAGGCAGTTTTTTT (High) SEQ ID NO: 38 Total Aerobic bacteria TTTTTTTTCCCTACGGGAGGCATTTTTTTT (Medium) SEQ ID NO: 39 Total Aerobic bacteria TTTATTTTCCCTACGGGAGGCTTTTATTTT (Low) SEQ ID NO: 47 Bile-tolerant Gram- TTTTTCTATGCAGTCATGCTGTGTGTRTGTCTTTTT negative (High) SEQ ID NO: 48 Bile-tolerant Gram- TTTTTCTATGCAGCCATGCTGTGTGTRTTTTTTT negative (Medium) SEQ ID NO: 49 Bile-tolerant Gram- TTTTTCTATGCAGTCATGCTGCGTGTRTTTTTTT negative (Low) SEQ ID NO: 53 Coliform/Enterobacteriaceae TTTTTTCTATTGACGTTACCCGCTTTTTTT SEQ ID NO: 81 stx1 gene TTTTTTCTTTCCAGGTACAACAGCTTTTTT SEQ ID NO: 82 stx2 gene TTTTTTGCACTGTCTGAAACTGCCTTTTTT SEQ ID NO: 59 etuf gene TTTTTTCCATCAAAGTTGGTGAAGAATCTTTTTT SEQ ID NO: 132 Negative control TTTTTTCTACTACCTATGCTGATTCACTCTTTTT SEQ ID NO: 65 Listeria spp. TTTTCTAAGTACTGTTGTTAGAGAATTTTT SEQ ID NO: 56 Aeromonas spp. TTATTTTCTGTGACGTTACTCGCTTTTATT SEQ ID NO: 78 Staphylococcus aureus 1 TTTATTTTCATATGTGTAAGTAACTGTTTTATTT SEQ ID NO: 49 Campylobacter spp. TTTTTTATGACACTTTTCGGAGCTCTTTTT SEQ ID NO: 72 Pseudomonas spp.3 TTTATTTTAAGCACTTTAAGTTGGGATTTTATTT SEQ ID NO: 53 Clostridium spp. TTTTCTGGAMGATAATGACGGTACAGTTTT SEQ ID NO: 42 Escherichia coli/ TTTTCTAATACCTTTGCTCATTGACTCTTT Shigella 1 SEQ ID NO: 74 Salmonella enterica/ TTTTTTTGTTGTGGTTAATAACCGATTTTT Enterobacter 1 SEQ ID NO: 61 invA gene TTTTTTTATTGATGCCGATTTGAAGGCCTTTTTT
(88) The set of 48 different probes of Table 4 were formulated as described in Table 3, then printed onto epoxysilane coated borosilicate glass, using an Gentics Q-Array mini contact printer with Arrayit SMP pins, which deposit about 1 nL of formulation per spot. As described in
Example 2
(89) Using the 3-Dimensional Lattice Microarray System for DNA Analysis
(90) Sample Processing
(91) Harvesting Pathogens from plant surface comprises the following steps:
(92) 1. Wash the plant sample or tape pull in 1× phosphate buffered saline (PBS)
(93) 2. Remove plant material/tape
(94) 3. Centrifuge to pellet cells & discard supernatant
(95) Resuspend in Sample Prep Buffer pre-mixed with Sample Digestion Buffer, sold under the trademark PathogenDx® and owned by PathogenDx, Inc.
(96) 5. Heat at 55° C. for 45 minutes
(97) 6. Vortex to dissipate the pellet
(98) 7. Heat at 95° C. for 15 minutes
(99) 8. Vortex and centrifuge briefly before use in PCR
(100) Amplification by PCR
(101) The sample used for amplification and hybridization analysis was a Cannabis flower wash from a licensed Cannabis lab. The washed flower material was then pelleted by centrifugation. The pellet was then digested with proteinaseK, then spiked with a known amount of Salmonella DNA before PCR amplification.
(102) TABLE-US-00005 TABLE 5 PCR Primers and PCR conditions used in amplification PCR primers (P1) for PCR Reaction #1 Cannabis ITS1 1° FP*-TTTGCAACAGCAGAACGACCCGTGA Cannabis ITS1 1° RP*-TTTCGATAAACACGCATCTCGATTG Enterobacteriaceae 16S 1° FP-TTACCTTCGGGCCTCTTGCCATCRGATGTG Enterobacteriaceae 16S 1° RP-TTGGAATTCTACCCCCCTCTACRAGACTCAAGC PCR primers (P2) for PCR Reaction #2 Cannabis ITS1 2° FP-TTTCGTGAACACGTTTTAAACAGCTTG Cannabis ITS1 2° RP-(Cy3)TTTTCCACCGCACGAGCCACGCGAT Enterobacteriaceae 16S 2° FP-TTATATTGCACAATGGGCGCAAGCCTGATG Enterobacteriaceae 16S 2° RP-(Cy3)TTTTGTATTACCGCGGCTGCTGGCA Primary PCR Secondary PCR PCR Reagent Concentration Concentration PCR Buffer 1X 2X MgCl.sub.2 2.5 mM 2.5 mM BSA 0.16 mg/mL 0.16 mg/mL dNTP's 200 mM 200 mM Prime mix 200 nM each 50 nM-FP/200 Taq Polymerase 1.5 Units 1.5 Units Program for PCR Reaction #1 95° C., 4 min 98° C., 30s 61° C., 30s 72° C., 60s 72° C., 7 min 25X Program for PCR Reaction #2 95° C., 4 min 98° C., 20s 61° C., 20s 72° C., 30s 72° C., 7 min 25X *FP, Forward Primer; *RP, Reverse Primer
(103) The Salmonella DNA spiked sample was then amplified with PCR primers (P1—Table 5) specific for the 16S region of Enterobacteriaceae in a tandem PCR reaction to first isolate the targeted region (PCR Reaction #1) and also PCR primers (P1—Table 5) which amplify a segment of Cannabis DNA (ITS) used as a positive control.
(104) The product of PCR Reaction #1 (14) was then subjected to a second PCR reaction (PCR Reaction #2) which additionally amplified and labelled the two targeted regions (16S, ITS) with green CY3 fluorophore labeled primers (P2—Table 5). The product of the PCR Reaction #2 (50 μL) was then diluted 1-1 with hybridization buffer (4×SSC+5×Denhardt's solution) and then applied directly to the microarray for hybridization.
(105) Hybridization
(106) Because the prior art method of microarray manufacture allows DNA to be analyzed via hybridization without the need for pre-treatment of the microarray
(107) surface, the use of the microarray is simple, and involves 6 manual or automated pipetting steps.
(108) 1) Pipette the amplified DNA+binding buffer onto the microarray
(109) 2) Incubate for 30 minutes to allow DNA binding to the microarray (typically at room temperature, RT)
(110) 3) Remove the DNA+binding buffer by pipetting
(111) 4) Pipette 50 uL of wash buffer onto the microarray (0.4×SSC+0.5×Denhardt's) and incubate 5 min at RT.
(112) 5) Remove the wash buffer by pipetting
(113) 6) Repeat steps 4&5
(114) 7) Perform image analysis at 532 nm and 635 nm to detect the probe spot location (532 nm) and PCR product hybridization (635 nm).
(115) Image Analysis
(116) Image Analysis was performed at two wavelengths (532 nm and 635 nm) on a raster-based confocal scanner: GenePix 4000B Microarray Scanner, with the following imaging conditions: 33% Laser power, 400 PMT setting at 532 nm/33% Laser Power, 700 PMT setting at 635 nm.
(117)
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Example 3
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(121)
(122) TABLE-US-00006 TABLE 6 First and Second PCR Primers SEQ ID NO. Primer target Primer sequence First PCR Primers (P1) for the first amplification step SEQ ID NO: 1 16S rDNA HV3 Locus TTTCACAYTGGRACTGAGACACG (Bacteria) SEQ ID NO: 2 16S rDNA HV3 Locus TTTGACTACCAGGGTATCTAATCCTGT (Bacteria) SEQ ID NO: 3 Stx1 Locus TTTATAATCTACGGCTTATTGTTGAACG (Pathogenic E. coli) SEQ ID NO: 4 Stx1 Locus TTTGGTATAGCTACTGTCACCAGACAATG (Pathogenic E. coli) SEQ ID NO: 5 Stx2 Locus TTTGATGCATCCAGAGCAGTTCTGCG (Pathogenic E. coli) SEQ ID NO: 6 Stx2 Locus TTTGTGAGGTCCACGTCTCCCGGCGTC (Pathogenic E. coli) SEQ ID NO: 7 InvA Locus (Salmonella) TTTATTATCGCCACGTTCGGGCAATTCG SEQ ID NO: 8 InvA Locus (Salmonella) TTTCTTCATCGCACCGTCAAAGGAACCG SEQ ID NO: 9 tuf Locus (All E. coli) TTTCAGAGTGGGAAGCGAAAATCCTG SEQ ID NO: 10 tuf Locus (All E. coli) TTTACGCCAGTACAGGTAGACTTCTG SEQ ID NO: 11 16S rDNA TTACCTTCGGGCCTCTTGCCATCRGATGTG Enterobacteriaceae HV3 Locus SEQ ID NO: 12 16S rDNA TTGGAATTCTACCCCCCTCTACRAGACTCAAGC Enterobacteriaceae HV3 Locus SEQ ID NO: 13 ITS2 Locus (All Yeast, TTTACTTTYAACAAYGGATCTCTTGG Mold/Fungus) SEQ ID NO: 14 ITS2 Locus (All Yeast, TTTCTTTTCCTCCGCTTATTGATATG Mold/Fungus) SEQ ID NO: 15 ITS2 Locus TTTAAAGGCAGCGGCGGCACCGCGTCCG (Aspergillus species) SEQ ID NO: 16 ITS2 Locus TTTTCTTTTCCTCCGCTTATTGATATG (Aspergillus species) SEQ ID NO: 17 ITS1 Locus TTTGCAACAGCAGAACGACCCGTGA (Cannabis/Plant) SEQ ID NO: 18 ITS1 Locus TTTCGATAAACACGCATCTCGATTG (Cannabis/Plant) Second PCR Primers (P2) for the second labeling amplification step SEQ ID NO: 19 16S rDNA HV3 Locus TTTACTGAGACACGGYCCARACTC (All Bacteria) SEQ ID NO: 20 16S rDNA HV3 Locus TTTGTATTACCGCGGCTGCTGGCA (All Bacteria) SEQ ID NO: 21 Stx1 Locus TTTATGTGACAGGATTTGTTAACAGGAC (Pathogenic E. coli) SEQ ID NO: 22 Stx1 Locus TTTCTGTCACCAGACAATGTAACCGCTG (Pathogenic E. coli) SEQ ID NO: 23 Stx2 Locus TTTTGTCACTGTCACAGCAGAAG (Pathogenic E. coli) SEQ ID NO: 24 Stx2 Locus TTTGCGTCATCGTATACACAGGAGC (Pathogenic E. coli) SEQ ID NO: 25 InvA Locus (All Salmonella) TTTTATCGTTATTACCAAAGGTTCAG SEQ ID NO: 26 InvA Locus (All Salmonella) TTTCCTTTCCAGTACGCTTCGCCGTTCG SEQ ID NO: 27 tuf Locus (All E. coli) TTTGTTGTTACCGGTCGTGTAGAAC SEQ ID NO: 28 tuf Locus (All E. coli) TTTCTTCTGAGTCTCTTTGATACCAACG SEQ ID NO: 29 16S rDNA TTATATTGCACAATGGGCGCAAGCCTGATG Enterbacteriaceae HV3 Locus SEQ ID NO: 30 16S rDNA TTTTGTATTACCGCGGCTGCTGGCA Enterbacteriaceae HV3 Locus SEQ ID NO: 31 ITS2 Locus (All Yeast, TTTGCATCGATGAAGARCGYAGC Mold/Fungus) SEQ ID NO: 32 ITS2 Locus (All Yeast, TTTCCTCCGCTTATTGATATGC Mold/Fungus) SEQ ID NO: 33 ITS2 Locus TTTCCTCGAGCGTATGGGGCTTTGTC (Aspergillus species) SEQ ID NO: 34 ITS2 Locus TITTTCCTCCGCTTATIGATATGC (Aspergillus species) SEQ ID NO: 35 ITS1 Locus TTTCGTGAACACGTTTTAAACAGCTTG (Cannabis/Plant) SEQ ID NO: 36 ITS1 Locus TTTCCACCGCACGAGCCACGCGAT (Cannabis/Plant)
(123)
(124)
(125)
(126)
(127)
(128)
(129) Table 7 displays representative oligonucleotide sequences which are used as microarray probes in an embodiment for DNA microarray-based analysis of bacterial 16S locus as described in
(130) Table 9 displays representative oligonucleotide sequences which are used as microarray probes in an embodiment for DNA microarray-based analysis of eukaryotic pathogens (fungi, yeast & mold) based on their ITS2 locus as described in
(131) Table 10 displays representative oligonucleotide sequences which are used as microarray probes in an embodiment for DNA microarray-based analysis of Cannabis at the ITS1 locus (Cannabis spp.).
(132) TABLE-US-00007 TABLE 7 Oligonucleotide probe sequence for the 16S Locus SEQ ID NO: 37 Total Aerobic bacteria TTTTTTTTTCCTACGGGAGGCAGTTTTTTT (High) SEQ ID NO: 38 Total Aerobic bacteria TTTTTTTTCCCTACGGGAGGCATTTTTTTT (Medium) SEQ ID NO: 39 Total Aerobic bacteria (Low) TTTATTTTCCCTACGGGAGGCTTTTATTTT SEQ ID NO: 40 Enterobacteriaceae TTTATTCTATTGACGTTACCCATTTATTTT (Low sensitivity) SEQ ID NO: 41 Enterobacteriaceae TTTTTTCTATTGACGTTACCCGTTTTTTTT (Medium sensitivity) SEQ ID NO: 42 Escherichia coli/Shigella 1 TTTTCTAATACCTTTGCTCATTGACTCTTT SEQ ID NO: 43 Escherichia coli/Shigella 2 TTTTTTAAGGGAGTAAAGTTAATATTTTTT SEQ ID NO: 44 Escherichia coli/Shigella 3 TTTTCTCCTTTGCTCATTGACGTTATTTTT SEQ ID NO: 45 Bacillus spp. Group1 TTTTTCAGTTGAATAAGCTGGCACTCTTTT SEQ ID NO: 46 Bacillus spp. Group2 TTTTTTCAAGTACCGTTCGAATAGTTTTTT SEQ ID NO: 47 Bile-tolerant Gram-negative TTTTTCTATGCAGTCATGCTGTGTGTRTGTCTTTTT (High) SEQ ID NO: 48 Bile-tolerant Gram-negative TTTTTCTATGCAGCCATGCTGTGTGTRTTTTTTT (Medium) SEQ ID NO: 49 Bile-tolerant Gram-negative TTTTTCTATGCAGTCATGCTGCGTGTRTTTTTTT (Low) SEQ ID NO: 50 Campylobacter spp. TTTTTTATGACACTTTTCGGAGCTCTTTTT SEQ ID NO: 51 Chromobacterium spp. TTTTATTTTCCCGCTGGTTAATACCCTTTATTTT SEQ ID NO: 52 Citrobacter spp. Group1 TTTTTTCCTTAGCCATTGACGTTATTTTTT SEQ ID NO: 53 Clostridium spp. TTTTCTGGAMGATAATGACGGTACAGTTTT SEQ ID NO: 54 Coliform/Enterobacteriaceae TTTTTTCTATTGACGTTACCCGCTTTTTTT SEQ ID NO: 55 Aeromonas TTTTTGCCTAATACGTRTCAACTGCTTTTT salmonicida/hydrophilia SEQ ID NO: 56 Aeromonas spp. TTATTTTCTGTGACGTTACTCGCTTTTATT SEQ ID NO: 57 Alkanindiges spp. TTTTTAGGCTACTGRTACTAATATCTTTTT SEQ ID NO: 58 Bacillus pumilus TTTATTTAAGTGCRAGAGTAACTGCTATTTTATT SEQ ID NO: 59 etuf gene TTTTTTCCATCAAAGTTGGTGAAGAATCTTTTTT SEQ ID NO: 60 Hafnia spp. TTTTTTCTAACCGCAGTGATTGATCTTTTT SEQ ID NO: 61 invA gene TTTTTTTATTGATGCCGATTTGAAGGCCTTTTTT SEQ ID NO: 62 Klebsiella oxytoca TTTTTTCTAACCTTATTCATTGATCTTTTT SEQ ID NO: 63 Klebsiella pneumoniae TTTTTTCTAACCTTGGCGATTGATCTTTTT SEQ ID NO: 64 Legionella spp. TTTATTCTGATAGGTTAAGAGCTGATCTTTATTT SEQ ID NO: 65 Listeria spp. TTTTCTAAGTACTGTTGTTAGAGAATTTTT SEQ ID NO: 66 Panteoa agglomerans TTTTTTAACCCTGTCGATTGACGCCTTTTT SEQ ID NO: 67 Panteoa stewartii TTTTTTAACCTCATCAATTGACGCCTTTTT SEQ ID NO: 68 Pseudomonas aeruginosa TTTTTGCAGTAAGTTAATACCTTGTCTTTT SEQ ID NO: 69 Pseudomonas cannabina TTTTTTTACGTATCTGTTTTGACTCTTTTT SEQ ID NO: 70 Pseudomonas spp. 1 TTTTTTGTTACCRACAGAATAAGCATTTTT SEQ ID NO: 71 Pseudomonas spp. 2 TTTTTTAAGCACTTTAAGTTGGGATTTTTT SEQ ID NO: 72 Pseudomonas spp. 3 TTTATTTTAAGCACTTTAAGTTGGGATTTTATTT SEQ ID NO: 73 Salmonella bongori TTTTTTTAATAACCTTGTTGATTGTTTTTT SEQ ID NO: 74 Salmonella TTTTTTTGTTGTGGTTAATAACCGATTTTT enterica/Enterobacter 1 SEQ ID NO: 75 Salmonella TTTTTTTAACCGCAGCAATTGACTCTTTTT enterica/Enterobacter 2 SEQ ID NO: 76 Salmonella TTTTTTCTGTTAATAACCGCAGCTTTTTTT enterica/Enterobacter 3 SEQ ID NO: 77 Serratia spp. TTTATTCTGTGAACTTAATACGTTCATTTTTATT SEQ ID NO: 78 Staphylococcus aureus 1 TTTATTTTCATATGTGTAAGTAACTGTTTTATTT SEQ ID NO: 79 Staphylococcus aureus 2 TTTTTTCATATGTGTAAGTAACTGTTTTTT SEQ ID NO: 80 Streptomyces spp. TTTTATTTTAAGAAGCGAGAGTGACTTTTATTTT SEQ ID NO: 81 stx1 gene TTTTTTCTTTCCAGGTACAACAGCTTTTTT SEQ ID NO: 82 stx2 gene TTTTTTGCACTGTCTGAAACTGCCTTTTTT SEQ ID NO: 83 Vibrio spp. TTTTTTGAAGGTGGTTAAGCTAATTTTTTT SEQ ID NO: 84 Xanthamonas spp. TTTTTTGTTAATACCCGATTGTTCTTTTTT SEQ ID NO: 85 Yersinia pestis TTTTTTTGAGTTTAATACGCTCAACTTTTT
(133) TABLE-US-00008 TABLE 8 Calibration and Negative Controls SEQ ID NO: 129 Imager Calibration TTTTCTATGTATCGATGTTGAGAAATTTTTTT (High) SEQ ID NO: 130 Imager Calibration TTTTCTAGATACTTGTGTAAGTGAATTTTTTT (Low) SEQ ID NO: 131 Imager Calibration TTTTCTAAGTCATGTTGTTGAAGAATTTTTTT (Medium) SEQ ID NO: 132 Negative control TTTTTTCTACTACCTATGCTGATTCACTCTTTTT
(134) TABLE-US-00009 TABLE 9 Oligonucleotide probe sequence for the ITS2 Locus SEQ ID NO: 86 Total Yeast and TTTTTTTTGAATCATCGARTCTTTGAACGCATTTTTTT Mold (High sensitivity) SEQ ID NO: 87 Total Yeast and TTTTTTTTGAATCATCGARTCTCCTTTTTTT Mold (Low sensitivity) SEQ ID NO: 88 Total Yeast and TTTTTTTTGAATCATCGARTCTTTGAACGTTTTTTT Mold (Medium sensitivity) SEQ ID NO: 89 Alternaria spp. TTTTTTCAAAGGTCTAGCATCCATTAAGTTTTTT SEQ ID NO: 90 Aspergillus flavus 1 TTTTTTCGCAAATCAATCTTTTTCCAGTCTTTTT SEQ ID NO: 91 Aspergillus flavus 2 TTTTTTTCTTGCCGAACGCAAATCAATCTTTTTTTTTTTT SEQ ID NO: 92 Aspergillus TTTCTTTTCGACACCCAACTTTATTTCCTTATTT fumigatus 1 SEQ ID NO: 93 Aspergillus TTTTTTTGCCAGCCGACACCCATTCTTTTT fumigatus 2 SEQ ID NO: 94 Aspergillus nidulans TTTTTTGGCGTCTCCAACCTTACCCTTTTT SEQ ID NO: 95 Aspergillus niger 1 TTTTTTCGACGTTTTCCAACCATTTCTTTT SEQ ID NO: 96 Aspergillus niger 2 TTTTTTTTCGACGTTTTCCAACCATTTCTTTTTT SEQ ID NO: 97 Aspergillus niger 3 TTTTTTTCGCCGACGTTTTCCAATTTTTTT SEQ ID NO: 98 Aspergillus terreus TTTTTCGACGCATTTATTTGCAACCCTTTT SEQ ID NO: 99 Blumeria TTTATTTGCCAAAAMTCCTTAATTGCTCTTTTTT SEQ ID NO: 100 Botrytis spp TTTTTTTCATCTCTCGTTACAGGTTCTCGGTTCTTTTTTT SEQ ID NO: 101 Candida albicans TTTTTTTTTGAAAGACGGTAGTGGTAAGTTTTTT SEQ ID NO: 102 Candida spp. TTTTTTTGTTTGGTGTTGAGCRATACGTATTTTT Group 1 SEQ ID NO: 103 Candida spp. TTTTACTGTTTGGTAATGAGTGATACTCTCATTTT Group 2 SEQ ID NO: 104 Chaetomium spp. TTTCTTTTGGTTCCGGCCGTTAAACCATTTTTTT SEQ ID NO: 105 Cladosporium spp TTTTTTTTGTGGAAACTATTCGCTAAAGTTTTTT SEQ ID NO: 106 Erysiphe spp. TTTCTTTTTACGATTCTCGCGACAGAGTTTTTTT SEQ ID NO: 107 Fusarium oxysporum TTTTTTTCTCGTTACTGGTAATCGTCGTTTTTTT SEQ ID NO: 108 Fusarium spp TTTTTTTTAACACCTCGCRACTGGAGATTTTTTT SEQ ID NO: 109 Golovinomyces TTTTTTCCGCTTGCCAATCAATCCATCTCTTTTT SEQ ID NO: 110 Histoplasma TTTATTTTTGTCGAGTTCCGGTGCCCTTTTATTT capsulatum SEQ ID NO: 111 Isaria spp. TTTATTTTTCCGCGGCGACCTCTGCTCTTTATTT SEQ ID NO: 112 Monocillium spp. TTTCTTTTGAGCGACGACGGGCCCAATTTTCTTT SEQ ID NO: 113 Mucor spp. TTTTCTCCAVVTGAGYACGCCTGTTTCTTTT SEQ ID NO: 114 Myrothecium spp. TTTATTTTCGGTGGCCATGCCGTTAAATTTTATT SEQ ID NO: 115 Oidiodendron spp. TTTTTTTGCGTAGTACATCTCTCGCTCATTTTTT SEQ ID NO: 116 Penicillium TTTTTTACACCATCAATCTTAACCAGGCCTTTTT oxalicum SEQ ID NO: 117 Penicillium paxilli TTTTTTCCCCTCAATCTTTAACCAGGCCTTTTTT SEQ ID NO: 118 Penicillium spp TTTTTTCAACCCAAATTTTTATCCAGGCCTTTTT SEQ ID NO: 119 Phoma/Epicoccum spp. TTTTTTTGCAGTACATCTCGCGCTTTGATTTTTT SEQ ID NO: 120 Podosphaera spp TTTTTTGACCTGCCAAAACCCACATACCATTTTT SEQ ID NO: 121 Podosphaera spp. TTTTTTTTAGTCAYGTATCTCGCGACAGTTTTTT SEQ ID NO: 122 Pythium oligandrum TTTTATTTAAAGGAGACAACACCAATTTTTATTT SEQ ID NO: 123 Rhodoturula spp TTTTTTCTCGTTCGTAATGCATTAGCACTTTTTT SEQ ID NO: 124 Stachybotrys spp TTTCTTCTGCATCGGAGCTCAGCGCGTTTTATTT SEQ ID NO: 125 Trichoderma spp TTTTTCCTCCTGCGCAGTAGTTTGCACATCTTTT
(135) Table 11 displays representative oligonucleotide sequences which are used as microarray probes in an embodiment for DNA microarray-based analysis of bacterial pathogens (stx1, stx2, invA, tuf) and for DNA analysis of the presence host Cannabis at the ITS1 locus (Cannabis spp.). It should be noted that this same approach, with modifications to the ITS1 sequence, could be used to analyze the presence of other plant hosts in such extracts.
(136) TABLE-US-00010 TABLE 10 Oligonucleotide probe sequence for the Cannabis ITS1 Locus SEQ ID NO: 126 Cannabis ITS1 DNA TTTTTTAATCTGCGCCAAGGAACAATATTTTTTT Control 1 SEQ ID NO: 127 Cannabis ITS1 DNA TTTTTGCAATCTGCGCCAAGGAACAATATTTTTT Control 2 SEQ ID NO: 128 Cannabis ITS1 DNA TTTATTTCTTGCGCCAAGGAACAATATTTTATTT Control 3
(137) TABLE-US-00011 TABLE 11 Representative Microarray Probe Design for the Present Invention: Bacterial Toxins, ITS1 (Cannabis) SEQ ID NO: 81 stx/gene TTTTTTCTTTCCAGGTACAACAGCTTTTTT SEQ ID NO: 82 stx2 gene TTTTTTGCACTGTCTGAAACTGCCTTTTTT SEQ ID NO: 59 etuf gene TTTTTTCCATCAAAGTTGGTGAAGAATCTTTTTT SEQ ID NO: 61 invA gene TTTTTTTATTGATGCCGATTTGAAGGCCTTTTTT SEQ ID NO: 126 Cannabis ITS1 DNA TTTTTTAATCTGCGCCAAGGAACAATATTTTTTT Control 1
(138)
(139)
(140)
(141)
(142) The data of
(143)
(144)
(145) Tables 12A and 12B show a collection of representative microarray hybridization data obtained from powdered dry food samples with no enrichment and 18-hour enrichment for comparison. The data shows that bacterial microbes were successfully detected on the microarrays of the present invention without the need for enrichment.
(146)
(147) If fresh leaf, flower, stem or root materials from fruit and vegetables are also washed in a water solution in that same way (when fresh, or after drying and grinding or other types or processing, then the present combination of RSG and microarray analysis would be capable of recovering and analyzing the DNA complement of those microbes in those other plant materials. At least two methods of sample collection are possible for fruit and vegetables. One method is the simple rinsing of the fruit, exactly as described for Cannabis, above. Another method of sample collection from fruits and vegetables is a “tape pull”, wherein a piece of standard forensic tape is applied to the surface of the fruit, then pulled off. Upon pulling, the tape is then soaked in the standard wash buffer described above, to suspend the microbes attached to the tape. Subsequent to the tape-wash step, all other aspects of the processing and analysis (i.e., raw sample genotyping, PCR, then microarray analysis) are exactly as described above.
(148) TABLE-US-00012 TABLE 12A Representative microarray data obtained from powdered dry food samples Sample Type Whey Protein Whey Protein Chewable Vanilla Pea Shake Vanilla Shake Chocolate Berry Tablet Shake Protein Enrichment time 0 18 0 18 0 18 0 18 0 18 hours hours hours hours hours hours hours hours hours hours Negative Control Probe 289 318 349 235 327 302 358 325 321 299 Total Aerobic Bacteria Probes High sensitivity 26129 38896 16629 11901 3686 230 32747 12147 41424 40380 Medium sensitivity 5428 6364 3308 2794 876 215 7310 2849 15499 8958 Low sensitivity 2044 3419 1471 990 446 181 2704 1062 4789 3887 Bile-tolerant Gram-negative Probes High sensitivity 2639 350 1488 584 307 305 1041 472 15451 8653 Medium sensitivity 1713 328 892 493 322 362 615 380 6867 4997 Low sensitivity 974 600 749 621 595 688 821 929 2459 1662 Total Enterobacteriaceae Probes High sensitivity 1131 306 363 310 346 318 273 331 4260 3149 Medium sensitivity 479 296 320 297 329 339 314 342 1489 990 Low sensitivity 186 225 203 165 205 181 207 200 216 259 16S rDNA Species Probes Escherichia coli/Shigella spp. 233 205 255 219 207 255 215 214 242 198 S. enterica/enterobacter spp. 203 183 186 281 212 299 197 257 308 303 Bacillus spp. 154 172 189 114 307 156 169 153 233 259 Pseudomonas spp. 549 201 202 251 148 216 303 276 2066 983 Organism Specific Gene Probes tuf gene(E. coli) 204 129 180 272 158 190 191 183 186 192 stx1 gene(E. coli) 241 178 171 240 289 304 195 245 149 191 stx2 gene(E. coli) 145 96 136 125 182 224 130 142 85 127 invA (Salmonella spp.) 215 265 210 284 204 256 239 285 237 229
(149) TABLE-US-00013 TABLE 12B Representative microarray data obtained from powdered dry food samples Sample Type Rice Work-out Work-out Vanilla Protein Shake FP Shake BR Shake Enrichment time 0 18 0 18 0 18 0 18 hours hours hours hours hours hours hours hours Negative Control Probe 351 351 271 309 299 332 246 362 Total Aerobic Bacteria Probes High sensitivity 471 288 17146 266 19207 261 41160 47198 Medium sensitivity 161 187 3120 229 3309 311 10060 22103 Low sensitivity 186 239 1211 261 1223 264 3673 6750 Bile-tolerant Gram-negative Probes High sensitivity 326 372 375 380 412 363 1418 358 Medium sensitivity 304 362 341 391 308 356 699 394 Low sensitivity 683 942 856 689 698 864 848 665 Total Enterobacteriaceae Probes High sensitivity 277 329 317 327 298 326 290 349 Medium sensitivity 326 272 296 291 297 263 262 307 Low sensitivity 215 207 204 288 213 269 195 247 16S rDNA Species Probes Escherichia coli/Shigella spp. 228 229 216 267 221 253 220 207 S. enterica/enterobacter spp. 226 281 238 268 197 254 255 216 Bacillus spp. 157 166 812 208 915 216 415 168 Pseudomonas spp. 199 225 247 251 211 259 277 225 Organism Specific Gene Probes tuf gene(E. coli) 150 149 126 206 163 212 215 166 stx1 gene(E. coli) 270 247 211 299 239 307 175 185 stx2 gene(E. coli) 158 178 127 205 138 175 128 100 invA (Salmonella spp.) 257 241 249 264 220 258 239 245
The data of Tables 13-15 demonstrates that simple washing of the fruit and tape pull sampling of the fruit generate similar microbial data. The blueberry sample is shown to be positive for Botrytis, as expected, since Botrytis is a well-known fungal contaminant on blueberries. The lemon sample is shown to be positive for Penicillium, as expected, since Penicillium is a well-known fungal contaminant for lemons.
(150) TABLE-US-00014 TABLE 13 Representative microarray hybridization data obtained from blueberry and lemon washes. Sample Blueberry Lemon Produce Wash Wash 1 blueberry in 2 ml Wash 1 piece moldy Collection Type 20 mM Borate, vortex 30 lemon in 2 ml 20 mM Protocol seconds Borate, vortex 30 seconds Dilution Factor NONE 1:20 NONE 1:20 A. fumigatus 1 65 61 62 57 A. fumigatus 2 66 61 58 131 A. fumigatus 3 69 78 55 127 A. fumigatus 4 80 198 63 161 A. fumigatus 5 98 68 59 70 A. flavus 1 111 65 197 58 A. flavus 2 64 66 71 49 A. flavus 3 72 79 54 49 A. flavus 4 95 71 66 125 A. flavus 5 59 55 45 47 A. niger 1 91 75 61 61 A. niger 2 185 68 61 57 A. niger 3 93 66 62 61 A. niger 4 1134 74 75 64 Botrytis spp. 1 26671 27605 60 55 Botrytis spp. 2 26668 35611 59 57 Penicillium spp. 1 63 69 2444 4236 Penicillium spp. 2 71 69 4105 7426 Fusarium spp. 1 175 69 59 78 Fusarium spp. 2 71 73 84 62 Mucor spp. 1 71 57 58 61 Mucor spp. 2 61 290 66 61 Total Y & M 1 20052 21412 8734 7335 Total Y & M 2 17626 8454 5509 5030
(151) TABLE-US-00015 TABLE 14 Representative microarray hybridization data obtained from blueberry washes and tape pulls Sample Moldy Blueberry Collection Type Tape Pull ID 1A1 1A1 1A2 1A2 1A3 1A3 1B1 1B1 1B2 1B2 1B3 1B3 Collection Point 1 500 ul 20 mM Borate Buffer, vortex 30 seconds 500 ul 20 mM Borate + Triton Buffer, vortex 30 seconds Collection Point 2 Add 15 mg zirconia beads, Add 15 mg zirconia beads, vortex, Heat 5 min 95° C., vortex, Heat 5 min 95° C., Vortex 15 seconds Vortex 15 seconds Collection Point 3 Heat 5 min Heat 5 min 95° C. vortex 95° C. vortex 15 seconds 15 seconds Dilution Factor NONE 1:20 NONE 1:20 NONE 1:20 NONE 1:20 NONE 1:20 NONE 1:20 A. fumigatus 1 66 388 83 77 97 313 95 68 76 55 75 60 A. fumigatus 2 97 100 82 118 69 56 87 67 185 76 58 52 A. fumigatus 3 77 94 82 1083 87 61 93 84 75 378 73 64 A. fumigatus 4 84 151 94 118 96 80 115 85 85 93 190 88 A. fumigatus 5 63 75 96 71 78 61 98 74 68 98 70 533 A. flavus 1 200 107 113 61 204 58 105 73 62 68 64 65 A. flavus 2 70 104 64 57 133 281 111 78 377 314 57 50 A. flavus 3 83 90 94 150 99 90 96 222 1162 86 80 73 A. flavus 4 76 125 92 146 87 174 241 78 115 69 105 85 A. flavus 5 80 153 77 72 78 439 71 86 280 58 62 57 A. niger 1 409 178 122 72 80 70 76 71 152 117 65 53 A. niger 2 78 292 79 65 715 666 74 70 68 731 70 54 A. niger 3 86 76 87 558 78 60 70 81 96 63 478 58 A. niger 4 164 70 92 108 197 69 130 75 76 148 73 65 Botrytis spp. 1 41904 26549 28181 29354 25304 25685 57424 33783 57486 49803 33176 32153 Botrytis spp. 2 36275 25518 29222 27076 26678 27675 49480 32899 52817 34322 29693 32026 Penicillium spp. 1 80 81 83 64 96 60 79 80 176 60 385 53 Penicillium spp. 2 90 93 81 80 114 59 98 69 470 65 478 56 Fusarium spp. 1 77 71 69 62 112 55 61 274 617 81 59 757 Fusarium spp. 2 91 82 107 74 101 65 91 66 123 63 71 583 Mucor spp. 1 90 314 73 88 105 61 77 79 741 180 172 74 Mucor spp. 2 83 69 73 69 91 67 111 102 455 88 70 133 Total Y & M 1 23637 18532 15213 17668 18068 19762 18784 15550 20625 17525 25813 18269 Total Y & M 2 12410 8249 9281 11526 8543 13007 14180 14394 9905 8972 15112 12678
The data embodied in
(152) TABLE-US-00016 TABLE 15 Representative microarray hybridization data obtained from lemon washes and tape pulls. Sample Moldy Lemon Collection Type Tape Pull ID 1A1 1A2 1A3 1B1 1B2 Lemon Lemon Lemon Lemon Lemon Collection Point 1 500 ul 20 mM Borate + Triton Buffer, vortex 30 seconds Collection Point 2 Add 15 mg Add 15 mg zirconia beads, zirconia beads, vortex, Heat 5 min vortex, Heat 5 min 95° C., Vortex 95° C., Vortex 15 seconds 15 seconds Collection Point 3 Heat 5 min 95° C. vortex 15 seconds Dilution Factor NONE A. fumigatus 1 96 83 75 83 64 A. fumigatus 2 221 73 71 66 101 A. fumigatus 3 87 88 85 92 122 A. fumigatus 4 83 85 91 72 97 A. fumigatus 5 448 100 84 114 78 A. flavus 1 85 79 70 66 63 A. flavus 2 77 82 77 79 63 A. flavus 3 133 66 86 60 67 A. flavus 4 96 85 81 98 88 A. flavus 5 68 62 65 106 59 A. niger 1 73 88 77 73 73 A. niger 2 74 84 81 71 103 A. niger 3 90 86 87 74 78 A. niger 4 82 93 104 86 161 Botrytis spp. 1 82 75 75 77 68 Botrytis spp. 2 91 74 83 67 62 Penicillium spp. 1 3824 5461 5500 4582 5290 Penicillium spp. 2 7586 8380 11177 6528 8167 Fusarium spp. 1 101 62 61 70 279 Fusarium spp. 2 77 122 78 68 233 Mucor spp. 1 74 110 89 76 57 Mucor spp. 2 132 1302 90 84 61 Total Y & M 1 8448 12511 9249 12844 8593 Total Y & M 2 9275 8716 11585 10758 4444
(153) Table 16 shows embodiments for the analysis of environmental water samples/specimens. The above teaching shows by example that unprocessed leaf and bud samples in Cannabis and hops may be washed in an aqueous water solution, to yield a water-wash containing microbial pathogens which can then be analyzed via the present combination of Raw Sample Genotyping (RSG) and microarrays. If a water sample containing microbes were obtained from environmental sources (such as well water, or sea water, or soil runoff or the water from a community water supply) and then analyzed directly, or after ordinary water filtration to concentrate the microbial complement onto the surface of the filter, that the present combination of RSG and microarray analysis would be capable of recovering and analyzing the DNA complement of those microbes.
(154) The data embodied in Table 16 were obtained from 5 well-water samples (named 2H, 9D, 21, 23, 25) along with 2 samples of milliQ laboratory water (obtained via reverse osmosis) referred to as “Negative Control”. All samples were subjected to filtration on a sterile 0.4 um filter. Subsequent to filtration, the filters, with any microbial contamination that they may have captured, were then washed with the standard wash solution, exactly as described above for the washing of Cannabis and fruit. Subsequent to that washing, the suspended microbes in wash solution were then subjected to exactly the same combination of centrifugation (to yield a microbial pellet) then lysis and PCR of the unprocessed pellet-lysate (exactly as described above for Cannabis), followed by PCR and microarray analysis, also as described for Cannabis.
(155) TABLE-US-00017 TABLE 16 Representative microarray data from raw water filtrate Sample ID Negative 2 H 2 H 9 D 9 D 21 21 23 23 25 25 Control Imager Calibration High 311 335 322 379 341 348 345 325 354 343 333 Imager Calibration Med 280 314 268 286 288 231 253 295 267 295 244 Imager Calibration Low 245 296 302 324 254 268 293 285 271 340 275 Cannabis cont. 310 330 313 255 323 368 313 322 274 332 322 Cannabis cont. 313 237 298 271 298 288 296 280 249 284 297 Cannabis cont. 208 265 276 250 267 327 255 258 253 282 370 Total Yeast & Mold 284 324 290 307 272 361 296 288 271 321 469 Total Yeast & Mold 251 259 294 290 309 308 285 281 275 299 293 Total Yeast & Mold 282 280 294 280 299 284 275 286 299 259 232 Total Aerobic bacteria High 40101 42007 47844 47680 45102 44041 43520 41901 46459 46783 135 Total Aerobic bacteria Medium 14487 12314 24189 26158 19712 16210 17943 15474 25524 18507 157 Total Aerobic bacteria Low 4885 5629 7625 6456 5807 4505 5316 6022 6264 6974 159 Negative Control 293 359 303 339 312 329 306 377 307 335 307 Aspergillus fumigatus 285 291 284 268 289 265 271 281 269 248 228 Aspergillus flavus 184 211 201 344 237 179 212 213 163 204 171 Aspergillus niger 226 213 228 273 190 195 245 206 222 209 172 Botrytis spp. 219 285 258 302 275 219 202 288 221 248 214 Alternaria spp. 81 97 76 89 58 76 75 175 117 174 167 Penicillium paxilli 135 162 215 142 127 161 103 115 238 190 200 Penicillium oxalicum 119 107 161 131 135 241 178 158 140 143 194 Penicillium spp. 50 123 179 177 128 138 146 163 148 115 184 Can. alb/trop/dub 261 236 235 230 250 213 276 244 245 237 194 Can. glab/Sach & Kluv spp. 146 165 196 128 160 215 185 217 215 177 225 Podosphaera spp. 111 119 100 122 192 105 95 43 169 27 143 Bile-tolerant Gram-negative High 16026 9203 13309 8426 16287 14116 10557 17558 15343 14285 183 Bile-tolerant Gram-negative Medium 12302 11976 9259 10408 13055 10957 11242 8416 9322 11785 196 Bile-tolerant Gram-negative Low 5210 7921 3818 3984 7224 6480 4817 6933 5021 5844 240 Total Enterobacteriaceae High 193 248 389 357 215 214 198 220 276 208 210 Total Enterobacteriaceae Med 246 214 297 246 244 224 219 245 252 229 207 Total Enterobacteriaceae Low 165 140 158 119 151 180 150 167 182 174 132 Total Coliform 121 148 158 117 129 117 155 157 125 178 152 Escherichia coli specific gene 31821 115 132 155 127 62 86 121 59 90 234 stx1 gene 67 0 2 0 0 23 21 28 0 0 116 stx2 gene 17 36 174 0 61 47 0 51 33 0 85 Salmonella specific gene 181 172 245 172 178 212 157 243 174 156 146 Bacillus spp. 137 135 174 112 164 143 163 182 168 152 149 Pseudomonas spp. 271 74 332 56 366 133 91 114 60 179 555 Escherichia coli/Shigella spp. 103 124 221 124 90 144 130 121 137 143 158 Salmonella enterica/enterobacter spp. 124 98 131 119 136 88 121 77 128 140 124 Erysiphe Group 2 278 221 237 230 245 254 250 220 205 236 233 Trichoderma spp. 105 157 204 152 180 154 130 161 201 180 150 Escherichia coli 429 431 551 576 549 406 407 484 556 551 293 Aspergillus niger 218 212 216 297 255 312 221 202 238 231 209 Escherichia coli/Shigella spp. 163 193 220 202 308 280 121 271 341 317 124 Aspergillus fumigatus 713 865 862 830 784 657 827 803 746 812 793 Aspergillus flavus 155 261 198 156 239 171 250 218 210 258 219 Salmonella enterica 136 98 85 43 109 47 23 123 70 100 135 Salmonella enterica 68 53 52 41 60 92 26 28 55 81 116
(156) The data seen in Table 16 demonstrate that microbes collected on filtrates of environmental water samples can be analyzed via the same combination of raw sample genotyping, then PCR and microarray analysis used for Cannabis and fruit washes. The italicized elements of Table 16 demonstrate that the 5 unprocessed well-water samples all contain aerobic bacteria and bile tolerant gram-negative bacteria. The presence of both classes of bacteria is expected for unprocessed (raw) well water. Thus, the data of Table 16 demonstrate that this embodiment of the present invention can be used for the analysis of environmentally derived water samples.
(157) The above teaching shows that unprocessed leaf and bud samples in Cannabis and hops may be washed in an aqueous water solution to yield a water-wash containing microbial pathogens which can then be analyzed via the present combination of RSG and microarrays. The above data also show that environmentally-derived well water samples may be analyzed by an embodiment. Further, if a water sample containing microbes were obtained from industrial processing sources (such as the water effluent from the processing of fruit, vegetables, grain, meat) and then analyzed directly, or after ordinary water filtration to concentrate the microbial complement onto the surface of the filter, that the present combination of RSG and microarray analysis would be capable of recovering and analyzing the DNA complement of those microbes.
(158) Further, if an air sample containing microbes as an aerosol or adsorbed to airborne dust were obtained by air filtration onto an ordinary air-filter (such as used in the filtration of air in an agricultural or food processing plant, or on factory floor, or in a public building or a private home) that such air-filters could then be washed with a water solution, as has been demonstrated for plant matter, to yield a microbe-containing filter eluate, such that the present combination of Raw Sample Genotyping (RSG) and microarray analysis would be capable of recovering and analyzing the DNA complement of those microbes.
(159) While the foregoing written description of an embodiments enables one of ordinary skill to make and use what is considered presently to be the best mode thereof, those of ordinary skill will understand and appreciate the existence of variations, combinations, and equivalents of the specific embodiment, method, and examples herein. The present disclosure should therefore not be limited by the above described embodiments, methods, and examples, but by all embodiments and methods within the scope and spirit of the present disclosure.