COMBINED SOLUTION PHASE AND SOLID PHASE DNA AMPLIFICATION

Abstract

Methods, systems, and apparatuses for efficiently amplifying and detecting certain nucleic acid sequences from a population. The selected population can be further characterised, for example by sequencing. A method involves combined solution phase and solid phase amplification.

Claims

1-24. (canceled)

25. A method for the amplification and analysis of nucleic acid sequences comprising: a. taking a system having a liquid volume in contact with a solid support wherein the liquid volume contains a nucleic acid sample, two or more non-immobilised amplification primers and reagents for nucleic acid amplification, and the solid support has one or more immobilised amplification primers; b. performing a nucleic acid amplification reaction using the non-immobilised amplification primers to produce a first non-immobilised nucleic acid amplification product; c. further amplifying the first non-immobilised nucleic acid amplification product using the one or more immobilised amplification primers to produce an immobilised second nucleic acid amplification product; d. either i. interrogating a localised signal generated at the immobilised second nucleic acid amplification product location in real time; or ii. removing the liquid volume and first non-immobilised amplification product and replacing with a new liquid volume having a primer which hybridises to the immobilised second nucleic acid amplification product, and either; 1. directly detecting the hybridised primer; or 2. flowing over the immobilised second amplification product a solution comprising at least one species of nucleotide in order to extend the hybridised primer, and e. detecting the presence, absence or sequence of the second nucleic acid amplification product.

26. The method according to claim 25 wherein the non-immobilised amplification primers in the liquid volume are released from the solid phase prior to amplification.

27. The method according to claim 25, wherein the nucleic acid amplification reaction using non-immobilised primers uses two or more pairs of non-immobilised primers.

28. The method according to claim 25, wherein the amplification is performed by thermocycling.

29. The method according to claim 25, wherein the nucleic acid amplification reaction using the non-immobilised primers is an isothermal amplification.

30. The method according to claim 29, wherein the second amplification product is produced by a further isothermal amplification.

31. The method according to claim 29, wherein the second amplification product is produced by thermocycling.

32. The method according to claim 25, wherein the amplification of the immobilised second nucleic acid amplification product is performed by interrogating a localised signal generated in real time.

33. The method according to claim 32, wherein the two primers in solution are present in different concentrations to give asymmetric amplification.

34. The method according to claim 25, wherein the primer hybridised to the second nucleic acid amplification product is fluorescently labelled.

35. The method according to claim 25, wherein the detection of the amplified products uses detection of the released protons from nucleotide incorporation.

36. The method according to claim 35, wherein the detection uses an ISFET sensor.

37. The method according to claim 25, wherein the detection of the amplified products involves fluorescent reporter probes and subsequent measurement of fluorescence.

38. The method according to claim 25, wherein the first and second amplification products are obtained using amplification primers having the same nucleic acid sequence.

39. The method according to claim 25, wherein the immobilised amplification primers amplify an internal section of the first amplification product such that the second amplification product is shorter than the first amplification product.

40. The method according to claim 25, wherein the first liquid volume is exposed to two or more immobilised amplification primers where each primer amplifies a different sequence.

41. The method according to claim 40, wherein the two or more immobilised amplification primers differ by a single base, thereby detecting single base variants in the first nucleic amplification products.

42. The method according to claim 40, wherein the immobilised primers are on an open microarray.

43. The method according to claim 40, wherein the immobilised primers are in separate wells.

44. A system for the amplification and detection of nucleic acid sequences comprising a liquid volume in contact with a solid support wherein the liquid volume contains a nucleic acid sample, one or more non-immobilised amplification primers and reagents for nucleic acid amplification, and the solid support has one or more immobilised amplification primers, wherein the system contains a sensor for detecting the amplification products.

45. The system according to claim 44, wherein the sensor is an optical sensor.

46. The system according to claim 44, wherein the sensor is an electrical sensor.

47. The system according to claim 44, wherein the sensor is a CMOS sensor.

48. A system according to claim 47, wherein the system contains multiple ISFET sensors and two or more immobilised primers, wherein each ISFET sensor contains a single immobilised primer.

Description

BRIEF DESCRIPTION OF THE DRAWINGS

[0031] FIG. 1: Schematic showing Single Localised Anchored Primer Amplification and Detection (LAPAD)

[0032] FIG. 2: Schematic showing Multiple Localised Anchored Primer Amplification and Detection (LAPAD)

[0033] FIG. 3: Schematic showing a run-off implementation. Takes place on an open system requiring flow capabilities on the chip. During the amplification reaction, product amplicon from the solution phase lands on the solid phase primers, which extend to create a forest of extended amplicon on the chip surface. Post amplification, the amplification product and reagents are washed away to leave single stranded amplicon on the chip surface. Run off primer and enzyme is loaded onto the chip, and, after a short hybridisation step, all four nucleotides are flowed in together, creating a burst of protons on those ISFETs with extended oligos. This proton burst is very clear to see with minimal data processing.

[0034] FIG. 4 shows a run-off workflow and data therefrom. The first row represents the amplification stage of the assay, generating a cluster of extended amplicon on the chip surface. This is followed by a dehybridisation step, using heat for example, to produce single stranded amplicon on the chip surface with no product in solution phase. Following hybridisation of the run off primer and enzyme, all four nucleotides are flowed across the chip and a signal is generated on those ISFETs which have been specifically extended.

[0035] FIG. 5 shows sample ISFET data showing run off signal generated following PCR for three target templates. Data shown is for E.coli (an 80 base product, therefore max 60 base run off), E. faecalis and S. marcescens following a specific amplification of the relevant target. Data is unmodified, with all ISFETs shown.

[0036] FIG. 6 shows a multiplexed chip spotted with three anchored primers and a positive template control. PCR with Ef template, followed by Run Off. Heat map shows ISFET voltage measured ˜15 seconds following nucleotide flow. ISFETs can be seen matching the spotting pattern and correspond to both Ef and positive control. Trace on the right shows examples of ISFET responses for each of the ISFET groups.

[0037] FIG. 7 shows a sequencing implementation. Rather than all four nucleotides add for the run-off, nucleotides are added sequentially. Takes place on an open system requiring flow capabilities on the chip. During the amplification reaction, product amplicon from the solution phase lands on the solid phase primers, which extend to create a forest of extended amplicon on the chip surface. Post amplification, the amplification product and reagents are washed away to leave single stranded amplicon on the chip surface. Sequencing primer and enzyme is loaded onto the chip, and, after a short hybridisation step, all four nucleotides are flowed in individually, creating a burst of protons on those ISFETs with amplification product and the correct template base. Single base resolution can be achieved.

[0038] FIG. 8 shows a sequencing workflow and data therefrom. The first row represents the amplification stage of the assay, generating a cluster of extended amplicon on the chip surface. This is followed by a dehybridisation step, using heat for example, to produce single stranded amplicon on the chip surface with no product in solution phase. Following hybridisation of the run off primer and enzyme, all four nucleotides are flowed individually across the chip and a signal is generated on those ISFETs where nucleotides were incorporated and corresponding to where amplification product was generated.

[0039] FIG. 9 shows a real-time detection workflow. Can take place on a platform with no fluid flow post chip amplification, or with minimal fluid flow. The reaction could take place in a permanently-sealed reaction chamber or chambers. During the amplification reaction, product amplicon from the solution phase lands on the solid phase oligos, modifying and extending the specific oligos. In a sealed system with low buffering, protons will be generated close to solid phase during the extension stage of each cycle of the amplification reaction. Pushing the asymmetry to give a significant excess of forward primer in the solution phase will effectively generate a “mini Run off” burst of protons in each cycle which should become detectable in the later cycles. An alternative to an asymmetry in the primers at the start of the amplification reaction, additional primer could be released or added during the amplification reaction, or at set time points. The amplification reaction will be in low buffer to allow real time detection of the pH signal.

[0040] FIG. 10 shows data from real-time detection. Chip spotted with multiple anchored primers in blocks, PCR (3:1 asymmetry) with 6 chamber gasket (3 chambers fluidically sealed), Run off in flow station with single chamber. Solution phase shows real time pH signal indicating that the reaction was progressing. As confirmation of amplification, post PCR, the chip was probed with a fluorescent label targeted against the distal end of the amplicon, and indicates that the anchored primers were extended during the PCR reaction.

[0041] FIG. 11 shows average delta signal from ISFETs for Example 1.

[0042] FIG. 12 shows delta signals from all ISFETS for Anchored Primer target Positive for Example 1.

[0043] FIG. 13 shows Delta signals from all ISFETs for Anchored Primer target Negative for Example 1.

[0044] FIG. 14 shows Delta signals from all ISFETs for Anchored Primer Control for Example 1.

[0045] FIG. 15 shows average ISFET signal results for Positive, Negative and Control primers for Example 1.

[0046] FIG. 16 is a gel electrophoresis image showing solution phase amplicon was generated post PCR for Serratia marcescens, for Example 1.

[0047] FIG. 17 shows a Sensospot fluorescent image for Example 1.

[0048] FIG. 18 shows average Delta signals from ISFETs for Example 2.

[0049] FIG. 19 shows Delta signals for Anchored Primers targets 1 to 4 Positive for Example 2.

[0050] FIG. 20 shows Delta signals from all ISFETs for Anchored Primer Negative for Example 2.

[0051] FIG. 21 shows Delta signals from all ISFETs for Anchored Primer Control for Example 2.

[0052] FIG. 22 shows average ISFET signal results for Positives, Negatives and Controls for Example 2.

[0053] FIG. 23 is a gel electrophoresis image for Example 2.

[0054] FIG. 24 is a Sensospot fluorescent image for Example 2.

DETAILED DESCRIPTION OF THE INVENTION

[0055] A system is described with the capability to generate a readout of different sequences from the same reaction volume.

[0056] Briefly, the system comprises a biphasic amplification reaction wherein a solution phase (PCR or isothermal) amplification reaction occurs in the presence of immobilised primers on the solid phase which further participate in producing amplification reaction product. The solution-phase (PCR or isothermal) amplification reaction can use one or more primers and target nucleic acid template to generate nucleic acid amplification product in solution with a corresponding signal being detected by the system when sufficient product has been produced. This solution-phase-generated nucleic acid amplification product, as well as the target nucleic acid template, can also act, or subsequently acts, as a template for an additional reaction on the solid phase whereby one or more immobilised primers interact with the solution-phase template as part of the amplification reaction and generate a nucleic acid sequence which is subsequently detectable by the system. By immobilising the primers in known locations and using a detection system capable of discriminating the location (for example, using ISFETs on CMOS IC chips or array type optical imaging systems) the readout enables the selective amplification and detection of many amplicons in the same device.

[0057] An amplification reaction is carried out in the solution phase in the presence of one or more further primers immobilised on the solid phase. The immobilised primers can be either the same sequence as one or more of the solution phase primers or correspond to internal sequences of the nucleic acid template generated in the solution phase. The former allows a second call to be made from the same reaction components, and the latter a second call that adds confirmation and increased confidence that the correct amplification reaction product has been generated and/or gives further information on the internal sequence of the target template.

[0058] The detection mode described herein can use ISFET CMOS technology but would also be applicable to existing nucleic acid amplification reactions and microarray methods, as well as a customised system to integrate the real time detection of both solution and solid phase reactions. The redundancy potential of the ISFET CMOS allows a significant number of replicates for each assay, as well as multiple target genes for each target, thereby improving the confidence in the system by relying upon multiple readouts for each target. Incorporation of positive and negative controls in each reaction vessel is also facilitated by this design, ensuring that correct calls are made when the control perform as required.

[0059] Below are various embodiments of the combined solution and solid phase amplification reaction.

[0060] DNA Amplification Readouts

[0061] The immobilised primers described can be the same as, or similar to, one or more of the solution phase primers, and participate in the amplification reaction such that an increased signal is generated from the immobilised primers when compared to an amplification carried out in the absence of the solution primers, thereby adding confidence in the result but without adding further information to the sequence being generated. For example, an asymmetric PCR in the solution phase can be compensated for by having the depleted primer in the solution phase present on the solid phase. As the amplification reaction progresses the solution phase product being generated is encouraged to interact with the solid phase, generating both solution phase and solid phase amplicons. The immobilised amplicon can be detected. Presence of this readout across multiple locations where the primer is immobilised gives increased confidence the then amplified material is definitely present in the sample. The confidence in the result is increased if immobilised primers having a different sequence do not give a positive result.

[0062] DNA Amplification with Internal Confirmation

[0063] The immobilised primers described can correspond to internal sequences of the DNA template generated in the solution phase such that any signal generated on the solid phase is positive confirmation that the correct product has been made in the solution phase. This confirmation demonstrates that the solution phase amplicon has not been generated by such things as primer dimers, mismatched primers or other non-specific reaction (for example, signals generated by interacting with the host (human) DNA when the intended target is a pathogen in the host sample), and gives a significant benefit over standard confirmatory tests such as melt curve analysis and electrophoresis gel imaging in that additional sequence information is inferred in the readout.

[0064] The internal confirmation signal is analogous to standard laboratory confirmatory procedures such as melt curve analysis, electrophoresis gel imaging, etc.

[0065] Using immobilised primers corresponding to internal sequences in the target template allows further specificity to be given to the system whereby the combination of solution phase reaction and solid phase reaction identifies more sequence information than a solution phase reaction on its own, thereby improving the confidence in the result compared to solution phase alone.

[0066] DNA Amplification with Internal Sequence Information

[0067] In addition to the confirmatory step already identified, the potential is also available to allow multiple immobilised primers to be present corresponding to different areas of the solution phase-amplified product, such that one or more can be used to provide internal information in addition to merely confirming that the correct product has been made in the solution phase.

[0068] This can take a simple form of multiple internal primers from the amplified product, each adding confidence in the inferred result by providing more than one sequence alignment, or in a more advanced version can be used to identify internal variations within a target gene corresponding to point mutations and other polymorphisms. For example, there are several antibiotic resistance genes which have multiple variants due to point mutations or other polymorphisms, and where the presence of a particular mutation may result in a different therapeutic strategy compared to another mutation. It is important, therefore, that identification of these polymorphisms is done in a timely and cost-effective manner. Current identification strategies using PCR and other amplification reactions are limited in capability and laboratories can resort to sequencing to elucidate the internal sequence and identify the polymorphisms—this is time-consuming and costly to implement and is often not done.

[0069] In this embodiment, a single primer pair can be used in the solution phase to amplify up all variants of the gene, with one or more immobilised primers corresponding to the point mutations or polymorphisms can be used on the solid phase to identify one or more of the variants. A combination of each of the internal immobilised primers provides the user with rich information on the overall sequence of the amplified gene and can result in clinical decisions being made easier and more quickly.

[0070] Run-Off (Including Multiple Run-Offs)

[0071] Amplification reactions are generally performed in high ionic strength buffers. For sequencing systems which measure the proton release of incorporated nucleotides, the amplification products can be detected if the amplification buffer is replaced by a buffer with a low buffering capacity. Alternatively the amplification products can be detected using fluorescently labelled primers or via the use of fluorescently labelled nucleotides.

[0072] The run-off takes place on an open system requiring flow capabilities on the chip. During the amplification reaction, product amplicon from the solution phase lands on the solid phase primers, which extend to create a forest of extended amplicon on the chip surface. Post amplification, the amplification product and reagents are washed away to leave single stranded amplicon on the chip surface. Run off primer and enzyme is loaded onto the chip, and, after a short hybridisation step, all four nucleotides are flowed in together, creating a burst of protons on those ISFETs with extended oligos. This proton burst is very clear to see with minimal data processing.

[0073] In order to perform an electronic/proton detection, at the end of the amplification stage described previously with both solution phase and solid phase reactions, the solution phase components are flushed out of the cartridge and replaced with a solution with low buffering capacity. This is then followed by primers and enzyme, either in sequence or combined, followed by a flow of nucleotides, which will result in a release of protons as the nucleotides are incorporated and a corresponding signal on the detection platform, for example a mV change on the relevant ISFETs. The primers used for the run-off can correspond to any location within the amplified template, including generic sequences added during earlier amplification reactions. Using amplicon specific primers internal to the solution amplified product delivers increased confidence in the result by confirming that the correct material has been made on the solid phase, but can add to the complexity of the system by having a higher multiplex. If generic sequences have been added in earlier amplification reactions, it would be possible to limit the scale of the solution phase multiplex thereby improving the efficiency of the reaction, however this may limit the readout confidence due to the potential for misfiring of the generic sequences.

[0074] By knowing the location of a particular immobilised primer, the identification of the target can be determined when the protons being generated during the run-off reaction result in a signal on the particular ISFET sensor to which the specific primer is immobilised. Multiple replicates for each assay target is possible in this embodiment, with the scale of the multiplex limited by spatial separation, the number of wells and sensors per device and bioinformatics challenges.

[0075] The system can make use of a single run-off reaction or multiple run-off reactions, with or without a dehybridisation step between each run. Additional run-offs can be used to interrogate the earlier signals such that increased confidence of the internal sequence can be made. For example, if generic sequences were used in earlier amplification reactions, a first run-off could use the generic sequence to identify which assays have generated signals, with subsequent run-off using specific primers corresponding to those particular assays to confirm that the correct product was made.

[0076] Multiple target sequences can be analysed in parallel as primers of different sequence can be immobilised in different locations on the solid support.

[0077] Sequence Information (Single or Multiple Bases at a Time)

[0078] At the end of the amplification stage described previously, the solution phase components can be flushed out of the cartridge and replaced with a solution with low buffering, as with the run-off workflow. This is then followed by primers and enzyme, either in sequence or combined, followed by a flow of individual nucleotides or combination of 2 or more nucleotides, which will result in a release of protons when the correct complementary nucleotides are flowed across the chip and incorporated. This workflow provides the richest information of all of the embodiments, in that it gives sequence information as opposed to relying only on the alignment of primers with their corresponding template. This workflow not only confirms that the correct alignment has taken place and the correct product has been made on the solid phase, but also indicates the internal sequence either by inference or by direct identification. Similar approaches can be used here as have been discussed in the run-off embodiment, with multiple runs being possible to provide further information, as well as a workflow that combines run-off with this approach of one or more nucleotides being used.

[0079] Real-Time Detection

[0080] The amplification process can be detected in real time by measuring the extension of the immobilised primers. The reaction could take place in a permanently-sealed reaction chamber or chambers. During the amplification reaction, product amplicon from the solution phase lands on the solid phase oligos, modifying and extending the specific oligos. In a sealed system with low buffering, protons will be generated close to solid phase during the extension stage of each cycle of the amplification reaction, and these can be detected.

[0081] The amplification can be asymmetric, where the two primers in solution are present in different concentrations, giving rise to amplification products which are largely single stranded due to the lack of a complementary primer to extend against them. Pushing the asymmetry to give a significant excess of forward primer in the solution phase will effectively generate a “mini Run off” burst of protons in each cycle which should become detectable in the later cycles. An alternative to an asymmetry in the primers at the start of the amplification reaction, additional primer could be released or added during the amplification reaction, or at set time points. The amplification reaction will be in low buffer to allow real time detection of the pH signal.

[0082] The source nucleic acid may be a genomic polynucleotide. The source material may be eukaryotic, prokaryotic, or archaeal. One or more source materials may be provided. The source nucleic acid may represent a fragment of a genome; for example, a single chromosome, or a single genomic locus (for example, for rapid sequencing of allelic polymorphisms). In particular examples the amplification may be specific for pathogenic material within a sample. For example the amplification may select bacterial or viral nucleic acids present within a human sample. Templates may be DNA, RNA, or the cDNA copies thereof.

[0083] The biological material may be amplified in solution prior to undergoing the claimed amplification reactions. Thus the material may already have undergone a step of sequence based amplification prior to the invention being performed. Alternatively the sample may be processed to attach a universal sequence common to one or both ends of all the strands in the sample. The universal sequence can be used as a universal sequence to hybridise to a common primer, which can be non-naturally occurring.

[0084] The invention described herein can allow for four or more levels of amplification specificity. A first amplification can be carried out in solution. A second amplification can be carried out using the non-immobilised primers. A third amplification can be carried out using immobilised primers of different sequence to the second amplification primers. The presence of the amplicon can be detected using a primer specific to the amplicon generated by the immobilised primers. Thus four levels of amplification specificity can be used, ensuring that the final amplicon is only detected if the originating sequence is absolutely definitely present in the sample. Thus false positive results from the detection of closely related, but undesired sequences can be eliminated.

[0085] Immobilisation of nucleic acids to surfaces is conventional. Any method of covalent or non covalent immobilisation may be used. The immobilisation is ideally stable to multiple cycles of thermocycling to a temperature causing nucleic acid strand separation. Particular methods of immobilisation include UV induced cross-linking or the immobilisation via the formation of amide bonds or phosphorothioate bonds.

EXAMPLES

[0086] Experimental data has been gathered for Single-Localised Anchored Primer Amplification and Detection (LAPAD) of Serratia marcescens (vendor: NCTC, catalogue number 27137) at a single target region and Multiple-Localised Anchored Primer Amplification and Detection (LAPAD) of Schizosaccharomyces pombe (vendor: ATCC, catalogue number: 26189) at multiple target regions.

[0087] Schematic representations of both Single and Multiple-LAPAD are shown as FIG. 1 and FIG. 2.

Example 1

Single Localised Anchored Primer Amplification and Detection (LAPAD)

[0088] Amplification and detection of Serratia marcescens at a single target region. The target region which is at the 3′ end of the amplified template DNA hybridised onto the complementary anchored primer target. During the amplification process this anchored primer target was extended and in the next stage the same target region was detected during extension. Primer/oligonucleotide sequences used are shown in Table 1.

TABLE-US-00001 TABLE 1 Oligonucleotide Sequences Oligonucleotide type Oligonucleotide name Sequence (5′.fwdarw.3′) Single LAPD Ser.marcescens_23s_F AGCCCAGAACCTGAATCG Excess primer Limiting primer Ser.marcescens_23s_R CCCTACTCATCGAACTCACG Anchored Primer target NH2_iSp18_SmR /5AmMC6//iSp18/CCCTACTCATCGAACTCACG Positive Anchored Primer Negative NH2_iSp18_SmIntRof /5AmMC6//iSp18/TGTGTGTTAGTGGAAGCGTC NH2_iSp18_EfR /5AmMC6//iSp18/GGGAGGTTCAGTTACTAACG NH2_iSp18_EfIntRof /5AmMC6//iSp18/GATCGTAAAACTCTGTTGTT Anchored Primer Control NH2_ddl_5′ + T15 /5AmMC6/TTTTTTTTTTTTTTTCGCGCTTCAATT CCTTGTTCAACGATTGCTCGAGAATCATACTGA TAGGCTGTTGCTAAAGCATTTTGCAGCTCTTCT CGGTTT Runoff Primer SM_IntRof_Cy3 /5Cy3/TGTGTGTTAGTGGAAGCGTC Multiple LAPAD Spom_gp_1_608_23_PAr TTCAGTGAGTTCTCCTGTTGATTG Excess primer Limiting primer Spom_gp_1_270_24_IDf AACGTTGGTATAGGAGAATGAAG Anchored Primer target 1 T10C10_iSp18_Spo_gp_1_ TTTTTTTTTTCCCCCCCCCC/isp18/AATACTATT Positive 338 + 19_5′_Rof AATATCACCTCAGTTTCAGCTGGGACTAATGAA Anchored Primer target 2 T10C10_iSp18_Spo_gp_1_ TTTTTTTTTTCCCCCCCCCC/isp18/GGGACTAAT Positive 369 + 24_5′_Rof GAATTGTTTTTACCTACTTTATCCCATGCTCAC G Anchored Primer target 3 T10C10_iSp18_Spo_gp_1_ TTTTTTTTTTCCCCCCCCCC/isp18/CCATACACA Positive 436 + 15_5′_Rof GACATAAGATATAACGGCTTCCCAGAACC Anchored Primer target 4 T10C10_iSp18_Spo_gp_1_ TTTTTTTTTTCCCCCCCCCC/isp18/GAGCATATT Positive 495 +20_5′_Rof ATCCTTTAATACCATTCGTTTAATCCCGTCCA Anchored Primer Negative T10C10_iSp18_Sa_nuc_1_ TTTTTTTTTTCCCCCCCCCC/isp18/AGTCTAAGT 186 + 19_Rof AGCTCAGCAAATGCATCACAAACAGATAACGG C T10C10_iSp18_Sa_nuc_1_ TTTTTTTTTTCCCCCCCCCC/isp18/GATAACGG 220 + 18_Rof CGTAAATAGAAGTGGTTCTGAAGATCCAACAG T T10C10_iSp18_Sa_nuc_1_ TTTTTTTTTTCCCCCCCCCC/isp18/TTAGACTAT 369 + 20_Rof TATTGGTTGATACACCTGAAACAAAGCATCCTA A T10C10_iSp18_Sa_nuc_1_ TTTTTTTTTTCCCCCCCCCC/isp18/AGGTGTAG 415 + 19_Rof AGAAATATGGTCCTGAAGCAAGTGCATTTACG AA Anchored Primer Control T10C10_ddl_5′-5 TTTTTTTTTTCCCCCCCCCCTTCAATTCCTTGTT CAACGATTGCTCGAGAATCATACTGATAGGCT GTTGCTAAAGCATTTTGCAGCTCTTCTCGGTTT Runoff Primer Spo_gp_1_578_23_Cy3P_RC /5Cy3/CTGCGCGTTTACCTACTTTGACT

Example 2

Multiple Localised Anchored Primer Amplification and Detection (LAPAD)

[0089] Amplification and detection of Schizosaccharomyces pombe at multiple target regions. Target region 1 which is after a few nucleotide bases from the 3′ end of the amplified template DNA hybridised onto the complementary anchored primer target 1. Target region 2 which after a few bases from target region 1 and towards the 5′ end of the amplified template DNA hybridised onto the complementary anchored primer target 2. Target region 3 which is after a few bases from target region 2 and towards the 5′ end of the amplified template DNA hybridised onto the complementary anchored primer target 3. Target region 4 which after a few bases from target region 3 and towards the 5′ end of the amplified template DNA hybridised onto the complementary anchored primer target 4. During the amplification process these 4 anchored primer targets with the hybridised DNA templates were extended and then in the next stage the same target regions were detected during extension. Primer/oligonucleotide sequences used are shown in Table 1.

[0090] Experimental Method

[0091] The chip platform incorporated ‘004’ Ta.sub.2O.sub.5 CMOS Chips consisting of ISFETs and enclosed in SU-8 wells were anchored with primers using a UV based cross-linking surface chemistry. A manifold was mounted onto the chip surface to include fluidics for the reaction to occur on the chip surface.

[0092] PCR was performed to generate DNA for detection, the PCR reagent recipe, final volume 50 μl , is shown in Table 2. Thermocycling conditions used are shown in Table 3.

TABLE-US-00002 TABLE 2 PCR Reagent Recipe Catalogue Reagent Vendor No. [Final] Units DNA free Roche 03315932001 — — Water 10X TITANIUM Clonetech 639209 1 X Taq PCR Buffer Potassium Sigma 60142 34 mM chloride Aldrich Betaine Sigma B0300 0.5 M Aldrich Bovine Serum Sigma B8667-5 ML 1 mg/mL Albumin Aldrich Glycerol Sigma G5516-100 ML 5 % Aldrich Triton X-100 Sigma T8787 0.1 % Aldrich dNTPs (each) Thermo R0186 0.06 mM Fisher Excess primer IDT Custom 0.5 μM Limiting primer IDT Custom 0.15 μM 50x TITANIUM Clonetech 639209 2.5 X Taq DNA Polymerase Genomic DNA See below See below 10,000 Copies/μL

TABLE-US-00003 TABLE 3 Thermocycling Conditions Temperature (° C.) Time (s) Cycles 95 60 1 95 5 40 59 10 72 5 95-60 2° C./minute 1 60 120 72 5

[0093] Post PCR, the chips were washed with wash buffer (0.06× Saline-Sodium Citrate, 0.06% Tween20), followed by chemical dehybridisation of DNA with 20 mM NaOH for 5 minutes and then washed with wash buffer again.

[0094] Runoff primer mix (sequence shown in Table 1) was then added to the chip surface. 3.33 μM of fluorescently labelled (Cy3) primer was added to Annealing buffer (5 mM Magnesium Acetate, 150 mM Sodium Chloride, 20 mM Tris pH 7.5, 0.01% Tween20).

[0095] The chips with the Runoff primer mix was then heated at 95° C. for 2minutes followed by 58° C. for 5minutes and left for incubation at room temperature for 15minutes. Chips were then washed with Enzyme loading buffer (1× Thermopol®, 0.06% Tween20).

[0096] Enzyme mix was then added onto the surface of the chip, this enzyme mix was created by adding 25units/μL of Custom made Bst Large Fragment DNA polymerase to Enzyme loading buffer. The chips were then incubated at room temperature for 5 minutes.

[0097] Deoxyribonucleotide triphosphate (dNTP) incorporation was achieved via use of a custom-made flow system enabling dNTPs to be flown on the chip surface. 12.5 μM each of Deoxyadenosine triphosphate, Deoxythymidine triphosphate, Deoxyguanosine triphosphate and Deoxycytidine triphosphate was added to non-carbonated RMD buffer (10 mM Magnesium Chloride, 25 mM Sodium Chloride, 0.025% Tergitol). The pH of the dNTP mix was adjusted to pH 8 and maintained by keeping the fluid under nitrogen gas.

[0098] ISFET Sensor Detection

[0099] The raw ISFET sensor voltage output data and Anchored primer spotting map was processed together by a custom data analysis pipeline (Galaxy Runoff pipeline v1.3.15).

[0100] Voltage signal peak heights from ISFETs were detected and Anchored primer ISFET voltage signal peak heights were subtracted from that of the adjacent upstream blank ISFET. This is done to remove system noise including noise from the fluidic flow which may mask detection. This delta ISFET sensor voltage output from all the specific Anchored primers sensors were averaged to determine signal detection.

[0101] E-Gel Electrophoresis Analysis

[0102] Readymade E-gels (48 well 2% agarose gels stained with Ethidium Bromide) were used for qualitative analysis of solution phase PCR. Samples were collected post PCR from the chip surface and 1 uL of the sample was adding to 1× E-gel loading dye before loading into the E-gel wells. A ladder was also loaded for size comparison of the amplicon. The gel was run for 10 minutes on the E-gel base which provides an electric field for the DNA amplicon to migrate according to its size.

[0103] Sensospot Fluorescence Imaging

[0104] Post run, chips were scanned in the Sensospot fluorescence scanner under a green light to illuminate the Cy3 runoff primer which would have hybridised onto the on-chip generated amplicon. Based on the fluorescence intensity, the on-chip amplification can be determined qualitatively.

[0105] Results

[0106] Detection for both assays was established quantitively by the delta ISFET sensor voltage output. The Solution phase PCR amplification was qualitatively assessed by E-gel analysis and Chip surface amplification by Sensospot fluorescent imaging.

Example 1

Single Localised Anchored Primer Amplification and Detection (LAPAD)

[0107] Target: Serratia marcescens

[0108] Chip ID: NM-248-0214

[0109] Anchored primer sequences for Example 1 can be seen in Table 4.

TABLE-US-00004 TABLE 4 Anchored Primer Sequences for Example 1 Anchored Primer target Positive NH2_iSp18_SmR Anchored Primer Negative NH2_iSp18_SmIntRof NH2_iSp18_EfR NH2_iSp18_EfIntRof Anchored Primer Control NH2_ddl_5′ + T15

[0110] Average delta signal from ISFETs can be seen in FIG. 11.

[0111] Delta signals from all ISFETs for Anchored Primer target Positive can be seen in FIG. 12.

[0112] Delta signals from all ISFETs for Anchored Primer target Negative can be seen in FIG. 13

[0113] Delta signals from all ISFETs for Anchored Primer control can be seen in FIG. 14.

[0114] Average ISFET signal results for Positive, Negative and Control primers can be seen in FIG. 15. An average 36.2 dmV ISFET signal was detected for the Positive Anchored primer NH2_iSp18_SmR which was even greater than the 23.4 dmV average ISFET signal for the Control Anchored Primer NH2_ddl_5′+T15.

[0115] Solution phase amplicon was generated post PCR for Serratia marcescens as seen in the gel electrophoresis image (FIG. 16). Along with the Control Anchored primer, the On-chip amplicon generated can also be seen for the Positive Anchored primer NH2-iSp18_SmR oil the sensospot fluorescent image (FIG. 17).

[0116] Amplification and detection of Serratia marcescetis at a single target region was demonstrated. A significant delta ISFET voltage signal was detected which was even larger than the Control Anchored Primer.

Example 2

Multiple Localised Anchored Primer Amplification and Detection (LAPAD)

[0117] Target: Schizosaccharomyces pombe

[0118] Chip ID: NM-248-0172

[0119] Anchored primer sequences for Example 2 can be seen in Table 5.

TABLE-US-00005 TABLE 5 Anchored primer sequences for Example 2. Anchored Primer T10C10_iSp18_Spo_gp_1_338 + 19_5′_Rof target 1 Positive Anchored Primer T10C10_iSp18_Spo_gp_1_369 + 24_5′_Rof target 2 Positive Anchored Primer T10C10_iSp18_Spo_gp_1_436 + 15_5′_Rof target 3 Positive Anchored Primer T10C10_iSp18_Spo_gp_1_495 + 20_5′_Rof target 4 Positive Anchored Primer T10C10_iSp18_Sa_nuc_1 _186 + 19_Rof Negative T10C10_iSp18_Sa_nuc_1 _220 + 18_Rof T10C10_iSp18_Sa_nuc_1 _369 + 20_Rof T10C10_iSp18_Sa_nuc_1 _415 + 19_Rof Anchored Primer T10C10_ddl_5′-5 Control

[0120] Average delta signal from ISFETs for Example 2, can be seen in FIG. 18. Delta signals from all ISFETs for Anchored Primer targets 1 to 4 Positive can be seen in FIG. 19.

[0121] Delta signals from all ISFETs for Anchored Primer Negative can be seen in FIG. 20.

[0122] Delta signals from all ISFETs for Anchored Primer Control can be seen in FIG. 21.

[0123] Average ISFET signal results for Positive, Negative and Control primers can be seen in FIGS. 22. 1.5 to 4.4 drnV ISFET signal was detected for the four Positive Anchored primers. This is much lower than previous signal intensities and the Control Anchored Primer average ISFET signal which was 34.6 dmV.

[0124] Solution phase amplicon was generated post PCR for Schizosaccharomyces pombe as seen in the gel electrophoresis image (FIG. 23). On-chip amplicon generated cannot be seen for the Positive Anchored primers on the sensospot fluorescent image (FIG. 24). The Control Anchored primer however can be seen.

[0125] Amplification and detection of Schizosaccharomyces pombe at multiple target regions was demonstrated.