WO2012131616A1 - Primer set, kit and methods thereof - Google Patents

Primer set, kit and methods thereof Download PDF

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Publication number
WO2012131616A1
WO2012131616A1 PCT/IB2012/051517 IB2012051517W WO2012131616A1 WO 2012131616 A1 WO2012131616 A1 WO 2012131616A1 IB 2012051517 W IB2012051517 W IB 2012051517W WO 2012131616 A1 WO2012131616 A1 WO 2012131616A1
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primers
primer
mutation
region
group
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PCT/IB2012/051517
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French (fr)
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Biswajit ROY
Kiran Venkatasubba HEGDE
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Chromous Biotech Pvt. Ltd.
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Publication of WO2012131616A1 publication Critical patent/WO2012131616A1/en

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    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
    • C12Q1/00Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
    • C12Q1/68Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving nucleic acids
    • C12Q1/6844Nucleic acid amplification reactions
    • C12Q1/6848Nucleic acid amplification reactions characterised by the means for preventing contamination or increasing the specificity or sensitivity of an amplification reaction
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
    • C12Q1/00Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
    • C12Q1/68Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving nucleic acids
    • C12Q1/6876Nucleic acid products used in the analysis of nucleic acids, e.g. primers or probes
    • C12Q1/6888Nucleic acid products used in the analysis of nucleic acids, e.g. primers or probes for detection or identification of organisms
    • C12Q1/689Nucleic acid products used in the analysis of nucleic acids, e.g. primers or probes for detection or identification of organisms for bacteria
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
    • C12Q1/00Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
    • C12Q1/68Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving nucleic acids
    • C12Q1/6844Nucleic acid amplification reactions
    • C12Q1/686Polymerase chain reaction [PCR]
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
    • C12Q2600/00Oligonucleotides characterized by their use
    • C12Q2600/16Primer sets for multiplex assays

Definitions

  • the present disclosure provides for a primer designing technique for amplification of templates with unpredicted sequence variations.
  • the present disclosure proposes a novel concept to design primers that can positively and accurately amplify targets from all strains/mutants of a microbe or an organism.
  • molecular diagnostic kits are available that rely on detection of presence of microbes / templates by PCR. Primers are designed and validated for the templates available across the country / region. Validations are required to ensure that there are no mismatches between the primer sequence and the primer annealing sequence within templates available in the Country / region. Further, even the kits developed and validated do not perform after few years as the organisms mutate over time.
  • a library of sequence data has to be generated and validated for developing consensus primers.
  • the microorganisms keep evolving / mutating continuously and more SNPs are introduced in their genome and thus, the consensus primers fail to amplify on PCRs over time.
  • the present disclosure relates to a primer set comprising plurality of primers having a maximum length N, ranging from about 19 to about 45 nucleotides, wherein each primer has a length selected from a group comprising N, N-1, N-2, N-3, N-4, N-5, N-6, N-7, N-8, N-9, N-10, N-l l , N-12, N-13, N-14, N-15, N-16, N-17, N-18, N-19, N- 20, N-21 , N-22, N-23, N-24, N-25 and N-26 or any combination thereof, wherein the primers are corresponding to a consensus sequence flanking a region of a target nucleotide sequence to be amplified, said region having mutation or suspected of having mutation at N th position; a kit for amplifying a region of target nucleotide sequence having mutation or suspected of having mutation at N th position, said kit having a primer set comprising plurality of primers having a maximum length N, ranging from about 19 to about
  • Figure 1 shows 4 strains which are indicated with minor variations / mutations within the region of primer annealing.
  • Figure 2 shows a comparative analysis between the present disclosure and prior art.
  • Figure 3 shows Amplicon from conventional PCR and PCR based on the present disclosure.
  • Figure 4 shows the results of PCR when the conventional primers are used (a) and the results of PCR when the primer set designed by the present disclosure are used (b).
  • Figure 5 shows the results of PCR when the conventional primers (fluorescent labeled) are used (a) and the results of PCR when the primer set (also fluorescent labeled) designed by the present disclosure are used (b).
  • the present disclosure relates to a primer set comprising plurality of primers having a maximum length N, ranging from about 19 to about 45 nucleotides, wherein each primer has a length selected from a group comprising N, N-l , N-2, N-3, N-4, N-5, N-6, N-7, N- 8, N-9, N-10, N-l l , N-l 2, N-l 3, N-14, N-15, N-16, N-l 7, N-18, N-l 9, N-20, N-21, N- 22, N-23, N-24, N-25 and N-26 or any combination thereof, wherein the primers are corresponding to a consensus sequence flanking a region of a target nucleotide sequence to be amplified, said region having mutation or suspected of having mutation at N position.
  • one of the primers in the set is having a length N and remaining primers in the set are having a length ranging from about N- 1 to about N-26 in any order thereof.
  • the present disclosure further relates to a kit for amplifying a region of target nucleotide sequence having mutation or suspected of having mutation at N th position, said kit having a primer set comprising plurality of primers having a maximum length N, ranging from about 19 to about 45 nucleotides, wherein each primer has a length selected from a group comprising N, N-l, N-2, N-3, N-4, N-5, N-6, N-7, N-8, N-9, N-10, N-l 1 , N-12, N-13, N- 14, N-15, N-16, N-17, N-18, N-19, N-20, N-21 , N-22, N-23, N-24, N-25 and N-26 or any combination thereof, wherein the primers are corresponding to a consensus sequence flanking said region, optionally along with DNA polymerase and nucleic acid amplification reagent selected from a group comprising magnesium chloride, dNTPs and buffer or any combination of reagents thereof;
  • the kit is a reaction mixture used for amplifying said region of the target nucleotide sequence.
  • the amplification is carried out by technique selected from a group comprising Conventional Polymerase Chain Reaction, HotStart Polymerase Chain Reaction, Real Time Polymerase Chain Reaction and Isothermal Amplifications.
  • the mutation is selected from a group comprising unpredicted sequence variations, SNPs, deletions, alternate splice products, microsatellites and gene rearrangements or any combination thereof.
  • the present disclosure further relates to a method of obtaining a primer set comprising plurality of primers having a maximum length N, ranging from about 19 to about 45 nucleotides, wherein each primer has a length selected from a group comprising N, N-l, N-2, N-3, N-4, N-5, N-6, N-7, N-8, N-9, N-10, N-l l, N-12, N-13, N-14, N-15, N-l 6, N- 17, N-l 8, N-l 9, N-20, N-21 , N-22, N-23, N-24, N-25 and N-26 or any combination thereof, said method comprising acts of: (a) identifying a region for amplification having mutation or suspected of having mutation at N th position in a target nucleotide sequence, followed by observing
  • the present disclosure further relates to a method of amplifying a region of target nucleotide sequence having mutation or suspected of having mutation at N th position, said method comprising act of subjecting the target nucleotide sequence to the reaction mixture as claimed above, for amplifying the said region.
  • the amplification with said reaction mixture provides amplified product of the mutated region.
  • the amplified product is detected by techniques selected from a group comprising Agarose based detection, spectrophotometric detection and fluorometric detection or any combination thereof.
  • primers of the reaction mixture amplifies said region of the target nucleotide sequence by binding to a consensus sequence flanking the region having mutation or suspected of having mutation at ⁇ ⁇ position.
  • primers of the reaction mixture anneal at same location at 3' end of the consensus sequence and at different locations at 5' end of the consensus sequence.
  • the amplification is carried out by technique selected from a group comprising Conventional Polymerase Chain Reaction, HotStart Polymerase Chain Reaction, Real Time Polymerase Chain Reaction and Isothermal Amplifications.
  • the mutation is selected from a group comprising unpredicted sequence variations, SNPs, deletions, alternate splice products, microsatellites and gene rearrangements or any combination thereof.
  • the target nucleotide sequence is selected from a group comprising prokaryotic and eukaryotic genomic sequence or a combination thereof.
  • the present disclosure provides for a novel concept to design primers for amplification of templates with probable variations/ mutations.
  • Primers are designed from data available from one strain / isolate that can positively and accurately amplify targets from all related strains irrespective of sequence variations. Further, development of series of primers and large-scale validation experiments will not be required and the PCR amplifications will work in spite of evolutionary changes or mutations. Hence, the present disclosure is a valuable tool to eliminate false negative cases in molecular diagnostics.
  • the present disclosure presents the following aspects:
  • a set of primers designed which amplifies the target sequence irrespective of whether there are mutations in the sequence where the primers anneal.
  • the primers are designed based on available information in public domains.
  • the primers (more than one forward primers in combination with more than one reverse primers) are used simultaneously for single reaction.
  • the primers are one or more bases smaller than each other. 6. Any one or more of the forward primer(s) would anneal on template and generate amplicons in combination with any one or more reverse primer(s).
  • the size of the amplicons is observed to be always identical irrespective of which set of the primers are used to amplify and give the amplicons.
  • kits The life of the kits will be prolonged. That means, once developed, the kits will be performing equally well over the years though the microbes / template might mutate over time.
  • the primers are designed based on reference sequence data available. b) Design 2 to 'N' sets of both forward and reverse primers each that anneal at identical regions on lower strand and upper strands respectively.
  • the forward primers are a combination of 2, 3 or more primers which are 1 , 2, 3 or more bases smaller than each other. It is the same for the reverse primer as well.
  • PCR always works even if there are mutations on the template within primer annealing sites. Further, the PCR products are detected by running samples on agarose gels (and run along with molecular weight markers for proper sizing) or by spectrophotometric / fiuorometric detection. POSSIBILITIES OF PRIMER SIZES / COMBINATIONS. RULES:
  • the second longest primer (forward & reverse) size can be smaller than 45 bases and can be till the point of a consensus region.
  • the third longest primer size (forward & reverse) can be smaller than the second longest primer and can be till the point of another consensus region.
  • the primers are used individually in combination of single forward and single reverse primer, the PCR reactions fail in case there are mutations in the last base (alone or in combination with other mutations spread around).
  • EXAMPLE 1 Schematic representation of sequence data for a targeted part of the template genome for PCR amplification
  • the figure 1 depicts 4 strains which are indicated with minor variations / mutations within the region of primer annealing and demonstrates how the primers would still anneal (and thus, PCR amplify) in spite of those mutations.
  • Primer- 1 BBB BBB BBB BBB BBB GAC TGA CTC AGT C Size: 28 bases
  • a wild template and a corresponding mutated template is generated in order to showcase the efficacy and success of amplification of the mutated template by the primers designed according to the present disclosure.
  • CF control forward
  • CR control reverse
  • WSP1FP (wild-type forward) primer is specific for wild type template and ends at G
  • Two tubes of PCR are set up with following combination of template and primers:
  • CF control forward
  • CR control reverse
  • Primer WSP1FP is specific to wild type template that ends at 'G'[N].
  • Primer WSP1-1FP is a base smaller that ends at 'G' [N-l].
  • Primer WSP1-2FP is 2 bases smaller that ends at 'C'[N-2].
  • Two tubes of PCR are set up with following combination of template and primers:
  • a wild template and a corresponding mutated template is generated in order to showcase the efficacy and success of amplification of the mutated template by the primers designed according to the present disclosure.
  • CRF Control Reverse Fluorescent primer is labeled at 5'- end with a fluorescent tag FAM (carboxy fluorescein) and,
  • WSP1FP (wild-type forward) primer is specific to wild type template (ends at G)
  • Two tubes of PCR are set up with following combination of template and primers:
  • PCR product After PCR, 1 micro litre of PCR product is taken in a vial and mixed with 8 micro litre of Formamide (Hi-DiTM Applied Biosystems, Part No. 431 1320) and 1 micro lit of Size Standard (Applied Biosystems, Part No.4322682) GeneScanTM -500 LIZ®. The mix is denatured 94 °C for 10 min and quick-chilled on ice.
  • Formamide Hi-DiTM Applied Biosystems, Part No. 431 1320
  • Size Standard Applied Biosystems, Part No.4322682
  • the quick chilled samples are loaded on the Genetic Analyzer (Applied Biosystems® 3500XL) and the samples are run and analyzed as per manufacturer's protocol.
  • CRF Control Reverse Fluorescent primer is labeled at 5'- end with a fluorescent tag FAM (carboxy fluorescein) and,
  • WSP1FP wild-type forward primer is specific to wild type template (ends at G)
  • Primer WSP1-1FP is a base smaller with respect to WSP1FP ends at 'G'
  • Primer WSP1-2FP is 2 bases smaller with respect to WSP1FP ends at 'C'.
  • Two tubes of PCR are set up with following combination of template and primers:
  • PCR product After PCR, 1 micro litre of PCR product is taken in a vial and mixed with 8 micro litre of Formamide (Hi-DiTM Applied Biosystems, Part No. 431 1320) and 1 micro lit of Size Standard (Applied Biosystems, Part No.4322682) GeneScanTM -500 LIZ®. The mix is denatured 94 °C for 10 min and quick-chilled on ice.
  • Formamide Hi-DiTM Applied Biosystems, Part No. 431 1320
  • Size Standard Applied Biosystems, Part No.4322682
  • the quick chilled samples are loaded on the Genetic Analyzer (Applied Biosystems® 3500XL) and the samples are electrophoresed and analyzed as per manufacturer's protocol.
  • primers there are 2 primers: one forward primer and one reverse primer.
  • the forward and reverse primers anneal on the template on the lower strand and upper strand respectively and amplify the region of the template between the annealing points.
  • Multiplex PCR protocols uses multiple sets/ pairs of primers that specifically and independently anneal at different regions on the template(s) and amplify multiple amplicons from the template(s). Also, each set of primer anneals specifically at the respective target template region only.
  • multiple sets of primers that specifically and independently anneal at the same region on the template and amplify the same amplicon from the template are used. Also, all or more than one primer sets can anneal the target template region and amplify the same.
  • step-wise PCR based protocol is for molecular diagnostic applications and the steps followed are provided below: 1.
  • Step- 1 Designing of primers .
  • Step-2 Isolation of sample target DNA.
  • Step-3 Performing PCR using standardized PCR cycle conditions using the primers, amplification reagents and sample target DNA.
  • Step-4 Detection of PCR product is carried by loading the product on Agarose gels.
  • PCR if PCR worked, it would indicate presence of the contamination/ infection. Failure of PCR suggests no contamination/ infection.
  • the most critical step within the 4 steps mentioned above is the designing of the primers (Step-1).
  • the primer sequences have to be chosen such that there are no mismatches between the template sequence and the primer sequence, particularly at the 3 '-end of the primer.
  • a primer set comprising a plurality of primers is designed based on the nucleotide sequence of the template and the possible mutated bases on the template as reported in the literature.
  • any one or more mismatches within the last 3 bases in the 3 '-end would result into sub- optimal or failure PCRs.
  • several sets of primers are usually designed for a particular organism/target and the performance of the primers is validated for all strains/variants available in the geographical region.
  • the size of an amplicon is the distance / size between the bases between the 5 '-ends of the forward and reverse primers used for PCR.
  • Figure-3 shows Amplicon from conventional PCR and PCR based on the present disclosure.
  • the PCR amplicon size is always the same as the 5 '-ends of both the primers (forward as well as reverse) end at identical points.
  • the current disclosure has applications in cancer detection as well as detection of genetic disorders apart from its applications to detect microbes. Some of the applications are captured below.
  • MDR Multiple Drug Resistance
  • Drug-resistant Malaria Drug-resistant Malaria
  • primers are designed for amplifying the hotspots (regions where most mutations occur) of the organism, it would serve 2 purposes; detection of the microbe as well as presence of mutations / MDR (detected by sequencing the amplicon).
  • Amplification of hotspots is possible through the current disclosure as it would allow PCR amplifications as NOT all 3 '-end positions of all primers would have mutations in the primer annealing regions.
  • Molecular diagnostic kits with primers designed as per the present disclosure would make the protocols fail-proof. At present, a PCR-based kit with a sensitivity of 90% is regarded as an "excellent" kit.

Abstract

The present disclosure provides for a primer designing for amplification of templates with unpredicted sequence variations. A major hurdle in designing primers for amplifications from microbial genomes is the presence of mutations, also called Single Nucleotide Polymorphisms (SNPs) among the microbial strains. One set of primer designed for PCR based detection of a particular strain of organism might fail to amplify another strain. To overcome this, multiple strains (nation-wide or globally) are sequenced and consensus / wobble primers are made. Furthermore, long-term validation programs continue as the microbes keep mutating continuously. The present disclosure proposes a novel concept to design primers that can positively and accurately amplify targets from all strains/mutants of a microbe or an organism.

Description

"PRIMER SET, KIT AND METHODS THEREOF" TECHNICAL FIELD
The present disclosure provides for a primer designing technique for amplification of templates with unpredicted sequence variations. The present disclosure proposes a novel concept to design primers that can positively and accurately amplify targets from all strains/mutants of a microbe or an organism.
BACKGROUND OF THE DISCLOSURE
Major hurdle in PCR amplification of any microbial genome is sequence variations (SNPs) within strains. Thus, a set of primers designed based on data obtained from one strain / isolate might fail to amplify the same target from another strain / isolate. To overcome these problems, large validation exercises are taken up to develop consensus primers.
Currently, molecular diagnostic kits are available that rely on detection of presence of microbes / templates by PCR. Primers are designed and validated for the templates available across the country / region. Validations are required to ensure that there are no mismatches between the primer sequence and the primer annealing sequence within templates available in the Country / region. Further, even the kits developed and validated do not perform after few years as the organisms mutate over time.
Some of the limitations of the existing technology:
1. A library of sequence data has to be generated and validated for developing consensus primers.
2. The microorganisms keep evolving / mutating continuously and more SNPs are introduced in their genome and thus, the consensus primers fail to amplify on PCRs over time.
3. Mismatch(es) at 3' end of primer annealing site (because of mutations introduced) can reduce PCR efficiency by 3-logs. (Reference: "Quantification of the
Detrimental Effect of a Single Primer-Template Mismatch by Real-Time PCR Using the 16S rR A Gene as an Example"; D. Bra, F. Martin-Laurent, and L. Philippot; APPLIED AND ENVIRONMENTAL MICROBIOLOGY; Mar. 2008, p. 1660-1663"). STATEMENT OF THE DISCLOSURE
Accordingly, the present disclosure relates to a primer set comprising plurality of primers having a maximum length N, ranging from about 19 to about 45 nucleotides, wherein each primer has a length selected from a group comprising N, N-1, N-2, N-3, N-4, N-5, N-6, N-7, N-8, N-9, N-10, N-l l , N-12, N-13, N-14, N-15, N-16, N-17, N-18, N-19, N- 20, N-21 , N-22, N-23, N-24, N-25 and N-26 or any combination thereof, wherein the primers are corresponding to a consensus sequence flanking a region of a target nucleotide sequence to be amplified, said region having mutation or suspected of having mutation at Nth position; a kit for amplifying a region of target nucleotide sequence having mutation or suspected of having mutation at Nth position, said kit having a primer set comprising plurality of primers having a maximum length N, ranging from about 19 to about 45 nucleotides, wherein each primer has a length selected from a group comprising N, N-1, N-2, N-3, N-4, N-5, N-6, N-7, N-8, N-9, N-10, N-11 , N-12, N-13, N- 14, N-15, N-16, N-17, N-18, N-19, N-20, N-21 , N-22, N-23, N-24, N-25 and N-26 or any combination thereof, wherein the primers are corresponding to a consensus sequence flanking said region, optionally along with DNA polymerase and nucleic acid amplification reagent selected from a group comprising magnesium chloride, dNTPs and buffer or any combination of reagents thereof; a method of obtaining a primer set comprising plurality of primers having a maximum length N, ranging from about 19 to about 45 nucleotides, wherein each primer has a length selected from a group comprising N, N-1, N-2, N-3, N-4, N-5, N-6, N-7, N-8, N-9, N-10, N-l l, N-12, N-13, N-14, N-15, N-16, N-17, N-18, N-19, N-20, N-21, N-22, N-23, N-24, N-25 and N-26 or any combination thereof, said method comprising acts of: (a) identifying a region for amplification having mutation or suspected of having mutation at Nth position in a target nucleotide sequence, followed by observing a consensus sequence flanking the said Nth position, and (b) synthesizing plurality of primers corresponding to the consensus sequence, wherein length of the primers range from about 19 to about 45 nucleotides to obtain said primer set; and a method of amplifying a region of target nucleotide sequence having mutation or suspected of having mutation at Nth position, said method comprising act of subjecting the target nucleotide sequence to the reaction mixture as claimed above, for amplifying the said region.
BRIEF DESCRIPTION OF ACCOMPANYING FIGURES
In order that the disclosure may be readily understood and put into practical effect, reference will now be made to exemplary embodiments as illustrated with reference to the accompanying figures. The figure together with a detailed description below, are incorporated in and form part of the specification, and serve to further illustrate the embodiments and explain various principles and advantages, in accordance with the present disclosure where:
Figure 1 shows 4 strains which are indicated with minor variations / mutations within the region of primer annealing.
Figure 2 shows a comparative analysis between the present disclosure and prior art.
Figure 3 shows Amplicon from conventional PCR and PCR based on the present disclosure.
Figure 4 shows the results of PCR when the conventional primers are used (a) and the results of PCR when the primer set designed by the present disclosure are used (b).
Figure 5 shows the results of PCR when the conventional primers (fluorescent labeled) are used (a) and the results of PCR when the primer set (also fluorescent labeled) designed by the present disclosure are used (b).
DETAILED DESCRIPTION
The present disclosure relates to a primer set comprising plurality of primers having a maximum length N, ranging from about 19 to about 45 nucleotides, wherein each primer has a length selected from a group comprising N, N-l , N-2, N-3, N-4, N-5, N-6, N-7, N- 8, N-9, N-10, N-l l , N-l 2, N-l 3, N-14, N-15, N-16, N-l 7, N-18, N-l 9, N-20, N-21, N- 22, N-23, N-24, N-25 and N-26 or any combination thereof, wherein the primers are corresponding to a consensus sequence flanking a region of a target nucleotide sequence to be amplified, said region having mutation or suspected of having mutation at N position.
In an embodiment of the present disclosure, one of the primers in the set is having a length N and remaining primers in the set are having a length ranging from about N- 1 to about N-26 in any order thereof.
The present disclosure further relates to a kit for amplifying a region of target nucleotide sequence having mutation or suspected of having mutation at Nth position, said kit having a primer set comprising plurality of primers having a maximum length N, ranging from about 19 to about 45 nucleotides, wherein each primer has a length selected from a group comprising N, N-l, N-2, N-3, N-4, N-5, N-6, N-7, N-8, N-9, N-10, N-l 1 , N-12, N-13, N- 14, N-15, N-16, N-17, N-18, N-19, N-20, N-21 , N-22, N-23, N-24, N-25 and N-26 or any combination thereof, wherein the primers are corresponding to a consensus sequence flanking said region, optionally along with DNA polymerase and nucleic acid amplification reagent selected from a group comprising magnesium chloride, dNTPs and buffer or any combination of reagents thereof;
In an embodiment of the present disclosure, the kit is a reaction mixture used for amplifying said region of the target nucleotide sequence.
In another embodiment of the present disclosure, the amplification is carried out by technique selected from a group comprising Conventional Polymerase Chain Reaction, HotStart Polymerase Chain Reaction, Real Time Polymerase Chain Reaction and Isothermal Amplifications.
In yet another embodiment of the present disclosure, the mutation is selected from a group comprising unpredicted sequence variations, SNPs, deletions, alternate splice products, microsatellites and gene rearrangements or any combination thereof. The present disclosure further relates to a method of obtaining a primer set comprising plurality of primers having a maximum length N, ranging from about 19 to about 45 nucleotides, wherein each primer has a length selected from a group comprising N, N-l, N-2, N-3, N-4, N-5, N-6, N-7, N-8, N-9, N-10, N-l l, N-12, N-13, N-14, N-15, N-l 6, N- 17, N-l 8, N-l 9, N-20, N-21 , N-22, N-23, N-24, N-25 and N-26 or any combination thereof, said method comprising acts of: (a) identifying a region for amplification having mutation or suspected of having mutation at Nth position in a target nucleotide sequence, followed by observing a consensus sequence flanking the said Νώ position, and (b) synthesizing plurality of primers corresponding to the consensus sequence, wherein length of the primers range from about 19 to about 45 nucleotides to obtain said primer set.
The present disclosure further relates to a method of amplifying a region of target nucleotide sequence having mutation or suspected of having mutation at Nth position, said method comprising act of subjecting the target nucleotide sequence to the reaction mixture as claimed above, for amplifying the said region.
In an embodiment of the present disclosure, the amplification with said reaction mixture provides amplified product of the mutated region.
In another embodiment of the present disclosure, the amplified product is detected by techniques selected from a group comprising Agarose based detection, spectrophotometric detection and fluorometric detection or any combination thereof.
In yet another embodiment of the present disclosure, primers of the reaction mixture amplifies said region of the target nucleotide sequence by binding to a consensus sequence flanking the region having mutation or suspected of having mutation at Νώ position.
In still another embodiment of the present disclosure, primers of the reaction mixture anneal at same location at 3' end of the consensus sequence and at different locations at 5' end of the consensus sequence. In still another embodiment of the present disclosure, the amplification is carried out by technique selected from a group comprising Conventional Polymerase Chain Reaction, HotStart Polymerase Chain Reaction, Real Time Polymerase Chain Reaction and Isothermal Amplifications.
In still another embodiment of the present disclosure, the mutation is selected from a group comprising unpredicted sequence variations, SNPs, deletions, alternate splice products, microsatellites and gene rearrangements or any combination thereof. In still another embodiment of the present disclosure, the target nucleotide sequence is selected from a group comprising prokaryotic and eukaryotic genomic sequence or a combination thereof.
The present disclosure provides for a novel concept to design primers for amplification of templates with probable variations/ mutations. Primers are designed from data available from one strain / isolate that can positively and accurately amplify targets from all related strains irrespective of sequence variations. Further, development of series of primers and large-scale validation experiments will not be required and the PCR amplifications will work in spite of evolutionary changes or mutations. Hence, the present disclosure is a valuable tool to eliminate false negative cases in molecular diagnostics.
The present disclosure presents the following aspects:
1. A set of primers designed which amplifies the target sequence irrespective of whether there are mutations in the sequence where the primers anneal.
2. The primers are designed based on available information in public domains.
3. The primers (more than one forward primers in combination with more than one reverse primers) are used simultaneously for single reaction.
4. All forward primers anneal at identical position in the 5 '-end but end at different positions at the 3 '-end.
5. The primers are one or more bases smaller than each other. 6. Any one or more of the forward primer(s) would anneal on template and generate amplicons in combination with any one or more reverse primer(s).
7. The size of the amplicons is observed to be always identical irrespective of which set of the primers are used to amplify and give the amplicons.
8. The concept would make "validation" requirements redundant which would be beneficial in the following ways:
a. No special knowledge of sequence is required.
b. Large expenses spent on Validation would be saved.
c. Long duration validation process can be avoided. Developmental processes will be faster.
d. The life of the kits will be prolonged. That means, once developed, the kits will be performing equally well over the years though the microbes / template might mutate over time.
THE PRIMER DESIGNING PROTOCOL:
a) The primers are designed based on reference sequence data available. b) Design 2 to 'N' sets of both forward and reverse primers each that anneal at identical regions on lower strand and upper strands respectively.
c) The forward primers are a combination of 2, 3 or more primers which are 1 , 2, 3 or more bases smaller than each other. It is the same for the reverse primer as well.
d) The forward primers' annealing position at the 5 '-end are identical but different at the 3'-end (Please refer to figure 1). It is the same for the reverse primers as well.
e) The primer-sets are mixed and PCR performed.
In an embodiment of the present disclosure, PCR always works even if there are mutations on the template within primer annealing sites. Further, the PCR products are detected by running samples on agarose gels (and run along with molecular weight markers for proper sizing) or by spectrophotometric / fiuorometric detection. POSSIBILITIES OF PRIMER SIZES / COMBINATIONS. RULES:
1. There can be more than one forward and more than one reverse primers for PCR.
2. Maximum length of the longest primer (forward & reverse): between 20 and 45 bases.
3. Minimum length of the smallest primer (forward & reverse): Between 19 and 44 bases.
4. The second longest primer (forward & reverse) size can be smaller than 45 bases and can be till the point of a consensus region.
5. Similarly, the third longest primer size (forward & reverse) can be smaller than the second longest primer and can be till the point of another consensus region.
6. All forward and reverse primers are mixed together and PCRs are performed.
7. In presence of mutations on template, while any one or more of primers fail to extend/ polymerize (because of mismatches between primer and template sequences), the other primers extend / polymerize to give PCR products. The same happens in case of mutations within both forward as well as reverse primer annealing positions.
Further, when the primers are used individually in combination of single forward and single reverse primer, the PCR reactions fail in case there are mutations in the last base (alone or in combination with other mutations spread around).
For example, if only the N-4 of Forward primer and only N-2 of Reverse primers are used in combination, the PCRs would fail in the following cases:
1. if there are mutations in 3 '-end positions (where the primer ends) on the forward primer annealing region.
2. if there are mutations in 3 '-end positions (where the primer ends) on the reverse primer annealing region.
The present disclosure is further elaborated with the help of following examples and associated figures. However, these examples should not be construed to limit the scope of the present disclosure. Further, as the scope of the present disclosure is non-limiting in nature, the instant primers can be applied to various other biotechnological applications such as but not limiting to those illustrated in the following examples. Further, all the possible amplification experiments involved in all such biotechnological applications fall under the purview of the present disclosure.
EXAMPLES
EXAMPLE 1: Schematic representation of sequence data for a targeted part of the template genome for PCR amplification
The figure 1 depicts 4 strains which are indicated with minor variations / mutations within the region of primer annealing and demonstrates how the primers would still anneal (and thus, PCR amplify) in spite of those mutations.
Assume only Strain A sequence is known while Strains B, C and D are variants present in nature.
Based on Strain-A sequence, the following primers are designed:
Primer- 1 : BBB BBB BBB BBB BBB GAC TGA CTC AGT C Size: 28 bases
(size = N)
Primer-2: BBB BBB BBB BBB BBB GAC TGA CTC AG Size: 26 bases (size = N-2)
Primer-3: BBB BBB BBB BBB BBB GAC TGA CTC Size: 24 bases (size = N-4) Where B is a base: A, T, G or C
All these three primers are used together in the PCR reaction and the observations are as follows:
For Strain A: all the 3 primers anneal and give the product.
For Strain B: Only Primer-2 and Primer-3 give product since Primer- 1 would fail as it has last base mismatch. For Strain C: Only Primer-2 and Primer-3 give product since Primer- 1 would fail as it has penultimate base mismatch.
For Strain D: Only Primer- 1 and Primer-3 give product since Primer-2 has penultimate base mismatch.
Use of all the three sets of primers together with N, N-2 and N-4 bases in size ensures that all mutant strains are amplified successfully and accurately.
EXAMPLE 2:
In an embodiment, a wild template and a corresponding mutated template is generated in order to showcase the efficacy and success of amplification of the mutated template by the primers designed according to the present disclosure.
Wild Template:
CTCACOCTOCTCGTTOAGTTTTGATTTTGCTGTTTCAAGCTCAACACGCAGTTT CCCTACTGTTAGCGCAATATCCTCGTTCTCCTGGTCGCGGCGTTTGATGTATT
Figure imgf000012_0001
TTTACTGATAAGTTCCAGATCCTCCTGGCAACTTGCACAAGTCCGACAACCCT
Figure imgf000012_0002
GCTGTAATTCTTCTATTTCTGATGCTGAATCAATGATGTCTGCCATC
Mutant Template: CTCACGCTGCTCGTTGAGTTTTGATTTTGCTGTTTCAAGCTCAACACGCAGTTT CCCTACTGTTAGCGCAATATCCTCGTTCTCCTGGTCGCGGCGTTTGATGTATT GCTGGTTTCTTTCCCGTTCATCCAGCAGTTCCAGCACAATCGATGGTGTTACC AATTCATGGAAAAGGTCTGCGTCAAATCCCCAGTCGTCATGCATTGCCTGCTC
TGCCGC?TTCACGCAGTGCCTGAGAGTTAATTTCGCTCACTTCGAACCTCTCTG TTTACTGATAAGTTCCAGATCCTCCTGGCAACTTGCACAAGTCCGACAACCCT GAACGACCAGGCGTCTTCGTTCATCTATCGGATCGCCACACTCACAACAATG AGTGGCAGATATAGCCTGGTGGTTCAGGCGGCGCATTTTTATTGCTGTGTTGC GCTGTAATTCTTCTATTTCTGATGCTGAATCAATGATGTCTGCCATC
Note: The bases mutated are in bold.
The following primers are designed to demonstrate the criticality of last base match on PCR efficiency:
Experiment 1:
Figure imgf000013_0002
Where, CF (control forward) and CR (control reverse) are Primers that amplify the 380 bp sequence containing the mutations and is used as PCR positive control.
WSP1FP (wild-type forward) primer is specific for wild type template and ends at G
Two tubes of PCR are set up with following combination of template and primers:
1. Wild template with CF,CR and WSP 1 FP primer.
2. Mutant template with CF,CR and WSP1FP primer. For the above two PCR reactions, following conditions with respect to the components are employed- Reaction Volume 25 μΐ
Enzyme FasTaq 0.25μ1 (0.75 Units)
Figure imgf000013_0001
PCR cycle conditions 94 °C 94 °C 55 °C 72 °C 72 °C 4 °C
2 min 5 sec 10 sec 1 sec 10 sec 00
1 Cycle 30 Cycles - ► 1 Cycle Hold
Observations [Figure 4 (a)]:
In lane 1, results for amplification of the wild-type template using the designed primers is shown. Both positive control primers (CF and CR) and WSP specific primers have worked, since the primers and template are perfectly complementary to each other.
In lane 2, results for amplification of the mutant template using the designed primers is shown. Only control primers (CF and CR) have worked and the WSP specific primers have failed, as the last base of the template is not complementary to the last base of the designed primer. Hence, no amplification occurs because of last base mismatch.
Experiment 2:
Figure imgf000014_0001
Where, CF (control forward) and CR (control reverse) are Primers that amplify the 380 bp sequence containing the mutations and is used as PCR positive control, and
Primer WSP1FP is specific to wild type template that ends at 'G'[N].
Primer WSP1-1FP is a base smaller that ends at 'G' [N-l].
Primer WSP1-2FP is 2 bases smaller that ends at 'C'[N-2]. Two tubes of PCR are set up with following combination of template and primers:
1. Wild template with CF,CR and WSP1FP, WSP1-1FP, WSP1-2FP primer mix.
2. Mutant template with CF,CR and WSP1FP WSP1-1FP, WSP1-2FP primer mix. For the above two PCR tubes, following conditions with respect to the components are employed-
Reaction Volume 25 μΐ
Enzyme FasTaq 0.25 μΐ (0.75 Units)
Figure imgf000015_0001
PCR cycle conditions
Figure imgf000015_0002
Observations [Figure 4 (b)]:
In lane 1, results for amplification of the wild-type template using the designed primers is shown. Both positive control primers (CF and CR) and WSP specific primers have worked since there are no mutations and thus all the primers bind and amplify the template.
In lane 2, results for amplification of the mutant template using the designed primers is shown. Both positive control primers (CF and CR) and WSP specific primers have worked. Therefore, it is observed that despite mutations in the template sequence, the designed consensus primer set [of Experiment 2] successfully amplifies the mutated template. A comparison of this experiment with experiment 1 above shows that primers having less bases [N-x] than [N] bases of the primer annealing region of the template are still able to successfully amplify even if the mutations are present at the Nth position. EXAMPLE 3:
In another embodiment, a wild template and a corresponding mutated template is generated in order to showcase the efficacy and success of amplification of the mutated template by the primers designed according to the present disclosure.
Wild Template:
CTCACGCTGCTCGTTGAGTTTTGATTTTGCTGTTTCAAGCTCAACACGCAGTTT CCCTACTGTTAGCGCAATATCCTCGTTCTCCTGGTCGCGGCGTTTGATGTATT
Figure imgf000016_0001
TTTACTGATAAGTTCCAGATCCTCCTGGCAACTTGCACAAGTCCGACAACCCT
Figure imgf000016_0002
GCTGTAATTCTTCTATTTCTGATGCTGAATCAATGATGTCTGCCATC
Mutant Template:
CTCACGCTGCTCGTTGAGTTTTGATTTTGCTGTTTCAAGCTCAACACGCAGTTT CCCTACTGTTAGCGCAATATCCTCGTTCTCCTGGTCGCGGCGTTTGATGTATT GCTGGTTTCTTTCCCGTTCATCCAGCAGTTCCAGCACAATCGATGGTGTTACC AATTCATGGAAAAGGTCTGCGTCAAATCCCCAGTCGTCATGCATTGCCTGCTC
TGCCGC?TTCACGCAGTGCCTGAGAGTTAATTTCGCTCACTTCGAACCTCTCTG
TTTACTGATAAGTTCCAGATCCTCCTGGCAACTTGCACAAGTCCGACAACCCT
GCTGTAATTCTTCTATTTCTGATGCTGAATCAATGATGTCTGCCATC The following primers are designed to demonstrate the criticality of last base match on PCR efficiency and how the present primer designing protocol overcomes it:
Experiment 1:
Figure imgf000017_0002
Where, CRF (Control Reverse Fluorescent) primer is labeled at 5'- end with a fluorescent tag FAM (carboxy fluorescein) and,
WSP1FP (wild-type forward) primer is specific to wild type template (ends at G)
Two tubes of PCR are set up with following combination of template and primers:
1. Wild template with CRF and WSP1FP primer.
2. Mutant template with CRF and WSP 1 FP primer.
For the above two PCR tubes, following conditions with respect to the components are employ ed-
Reaction Volume 25 μΐ
Enzyme FasTaq 0.25 μΐ (0.75 Units)
Figure imgf000017_0001
PCR cycle conditions
Figure imgf000017_0003
After PCR, 1 micro litre of PCR product is taken in a vial and mixed with 8 micro litre of Formamide (Hi-DiTM Applied Biosystems, Part No. 431 1320) and 1 micro lit of Size Standard (Applied Biosystems, Part No.4322682) GeneScan™ -500 LIZ®. The mix is denatured 94 °C for 10 min and quick-chilled on ice.
The quick chilled samples are loaded on the Genetic Analyzer (Applied Biosystems® 3500XL) and the samples are run and analyzed as per manufacturer's protocol.
Observations [Figure 5 (a)]:
In Lane -A, results for amplification of the wild-type template using the designed primers is shown. Peak seen at 184 bp indicates successful PCR. Hence, both positive control primer and WSP specific primer have worked since there are no mutations and thus all the primers bind and amplify the template.
In Lane-B, results for amplification of the mutant template using the designed primers is shown. No peak is seen indicating failure of PCR due to last base mismatch in the mutant template. The WSP specific primers have failed, as the last base is not complementary to the last base of the designed primer. Hence, no amplification occurs because of last base mismatch. Experiment 2:
Figure imgf000018_0001
Where, CRF (Control Reverse Fluorescent) primer is labeled at 5'- end with a fluorescent tag FAM (carboxy fluorescein) and,
WSP1FP (wild-type forward) primer is specific to wild type template (ends at G), Primer WSP1-1FP is a base smaller with respect to WSP1FP ends at 'G', Primer WSP1-2FP is 2 bases smaller with respect to WSP1FP ends at 'C'.
Two tubes of PCR are set up with following combination of template and primers:
1. Wild template with CRF and WSP1FP primer.
2. Mutant template with CRF and WSP1FP primer mix.
For the above two PCR tubes, following conditions with respect to the components employed-
Reaction Volume 25 μΐ
Enzyme FasTaq 0.25 μΐ (0.75 Units)
Figure imgf000019_0001
PCR cycle conditions
Figure imgf000019_0002
After PCR, 1 micro litre of PCR product is taken in a vial and mixed with 8 micro litre of Formamide (Hi-DiTM Applied Biosystems, Part No. 431 1320) and 1 micro lit of Size Standard (Applied Biosystems, Part No.4322682) GeneScan™ -500 LIZ®. The mix is denatured 94 °C for 10 min and quick-chilled on ice.
The quick chilled samples are loaded on the Genetic Analyzer (Applied Biosystems® 3500XL) and the samples are electrophoresed and analyzed as per manufacturer's protocol.
Observations [Figure 5 (b)l:
In Lane-C, results for amplification of the wild-type template using the designed primers is shown. Peak is seen at 184 bp indicating successful PCR. Both positive control primer and WSP specific primers have worked since there are no mutations and thus all the primers bind and amplify the template. .
In Lane-D, results for amplification of the mutant template using the designed primers is shown. Peak is seen at 184 bp indicating successful PCR due to employment of novel primer set. Both positive control primer and WSP specific primers have worked. Therefore, it is observed that despite mutations in the template sequence, the designed consensus primer set [of Experiment 2] successfully amplifies the mutated template. A comparison of this experiment with experiment 1 above shows that primers having less bases [N-x] than [N] bases of the primer annealing region of the template are still able to successfully amplify even if the mutations are present at the Nth position.
EXAMPLE 4:
In regular PCRs, there are 2 primers: one forward primer and one reverse primer. The forward and reverse primers anneal on the template on the lower strand and upper strand respectively and amplify the region of the template between the annealing points.
Conventionally, Multiplex PCR protocols uses multiple sets/ pairs of primers that specifically and independently anneal at different regions on the template(s) and amplify multiple amplicons from the template(s). Also, each set of primer anneals specifically at the respective target template region only.
In the present disclosure, multiple sets of primers that specifically and independently anneal at the same region on the template and amplify the same amplicon from the template are used. Also, all or more than one primer sets can anneal the target template region and amplify the same.
EXAMPLE 5:
STEP-WISE PCR-BASED PROTOCOL
In an embodiment the step-wise PCR based protocol is for molecular diagnostic applications and the steps followed are provided below: 1. Step- 1 : Designing of primers .
2. Step-2: Isolation of sample target DNA.
3. Step-3: Performing PCR using standardized PCR cycle conditions using the primers, amplification reagents and sample target DNA.
4. Step-4: Detection of PCR product is carried by loading the product on Agarose gels.
Finally, if PCR worked, it would indicate presence of the contamination/ infection. Failure of PCR suggests no contamination/ infection. The most critical step within the 4 steps mentioned above is the designing of the primers (Step-1). The primer sequences have to be chosen such that there are no mismatches between the template sequence and the primer sequence, particularly at the 3 '-end of the primer. In an exemplary embodiment, a primer set comprising a plurality of primers is designed based on the nucleotide sequence of the template and the possible mutated bases on the template as reported in the literature.
Any one or more mismatches within the last 3 bases in the 3 '-end would result into sub- optimal or failure PCRs. Thus, several sets of primers are usually designed for a particular organism/target and the performance of the primers is validated for all strains/variants available in the geographical region.
EXAMPLE 6:
This example provides for a comparative analysis between the present disclosure and prior art; depicting the absence of amplification when mutations are present in the template in prior art studies and on the other hand irrespective of the presence of mutations the amplification of the template in the instant disclosure [Figure 2].
EXAMPLE 7:
The size of an amplicon is the distance / size between the bases between the 5 '-ends of the forward and reverse primers used for PCR. Figure-3 shows Amplicon from conventional PCR and PCR based on the present disclosure. The PCR amplicon size is always the same as the 5 '-ends of both the primers (forward as well as reverse) end at identical points.
The current disclosure has applications in cancer detection as well as detection of genetic disorders apart from its applications to detect microbes. Some of the applications are captured below.
1. Multiple Drug Resistance (MDR) Tuberculosis, Drug-resistant Malaria, Methicilin Resistant Staphylococcus aureus (MRSA), etc, occur when mutations are introduced within genes responsible for drug resistance.
2. Thus, if primers are designed for amplifying the hotspots (regions where most mutations occur) of the organism, it would serve 2 purposes; detection of the microbe as well as presence of mutations / MDR (detected by sequencing the amplicon).
3. Amplification of hotspots is possible through the current disclosure as it would allow PCR amplifications as NOT all 3 '-end positions of all primers would have mutations in the primer annealing regions.
Advantages:
a. Molecular diagnostic kits with primers designed as per the present disclosure would make the protocols fail-proof. At present, a PCR-based kit with a sensitivity of 90% is regarded as an "excellent" kit.
b. Over-all success rate (in terms of sensitivity and specificity) for molecular diagnostics will improve resulting in better acceptance of the molecular protocols. c. Molecular diagnostic kit development programs will benefit as large scale validation process will not be required.

Claims

We Claim:
1. A primer set comprising plurality of primers having a maximum length N, ranging from about 19 to about 45 nucleotides, wherein each primer has a length selected from a group comprising N, N-l, N-2, N-3, N-4, N-5, N-6, N-7, N-8, N- 9, N-10, N-l l, N-12, N-l 3, N-l 4, N-15, N-16, N-17, N-18, N-l 9, N-20, N-21 , N- 22, N-23, N-24, N-25 and N-26 or any combination thereof, wherein the primers are corresponding to a consensus sequence flanking a region of a target nucleotide sequence to be amplified, said region having mutation or suspected of having mutation at Nth position.
2. The primer set as claimed in claim 1, wherein one of the primers in the set is having a length N and remaining primers in the set are having a length ranging from about N- 1 to about N-26 in any order thereof.
3. A kit for amplifying a region of target nucleotide sequence having mutation or suspected of having mutation at Nth position, said kit having a primer set comprising plurality of primers having a maximum length N, ranging from about 19 to about 45 nucleotides, wherein each primer has a length selected from a group comprising N, N-l, N-2, N-3, N-4, N-5, N-6, N-7, N-8, N-9, N-10, N-l l, N-12, N-13, N-14, N-15, N-16, N-17, N-18, N-l 9, N-20, N-21 , N-22, N-23, N-24, N-25 and N-26 or any combination thereof, wherein the primers are corresponding to a consensus sequence flanking said region, optionally along with DNA polymerase and nucleic acid amplification reagent selected from a group comprising magnesium chloride, dNTPs and buffer or any combination of reagents thereof.
4. The kit as claimed in claim 3, wherein the kit is a reaction mixture used for amplifying said region of the target nucleotide sequence.
5. The primer set as claimed in claim 1 and the kit as claimed in claim 3, wherein the amplification is carried out by technique selected from a group comprising Conventional Polymerase Chain Reaction, HotStart Polymerase Chain Reaction, Real Time Polymerase Chain Reaction and Isothermal Amplifications.
6. The primer set as claimed in claim 1 and the kit as claimed in claim 3, wherein the mutation is selected from a group comprising unpredicted sequence variations, SNPs, deletions, alternate splice products, microsatellites and gene rearrangements or any combination thereof.
7. A method of obtaining a primer set comprising plurality of primers having a maximum length N, ranging from about 19 to about 45 nucleotides, wherein each primer has a length selected from a group comprising N, N-l, N-2, N-3, N-4, N-5,
N-6, N-7, N-8, N-9, N-10, N-l l , N-12, N-13, N-l 4, N-l 5, N-16, N-l 7, N-18, N- 19, N-20, N-21 , N-22, N-23, N-24, N-25 and N-26 or any combination thereof, said method comprising acts of:
a. identifying a region for amplification having mutation or suspected of having mutation at Nth position in a target nucleotide sequence, followed by observing a consensus sequence flanking the said ώ position; and b. synthesizing plurality of primers corresponding to the consensus sequence, wherein length of the primers range from about 19 to about 45 nucleotides to obtain said primer set.
8. A method of amplifying a region of target nucleotide sequence having mutation or suspected of having mutation at Nth position, said method comprising act of subjecting the target nucleotide sequence to the reaction mixture as claimed in claim 4, for amplifying the said region.
9. The method as claimed in claim 8, wherein the amplification with said reaction mixture provides amplified product of the mutated region.
10. The method as claimed in claim 9, wherein the amplified product is detected by techniques selected from a group comprising Agarose based detection, spectrophotometric detection and fluorometric detection or any combination thereof.
11. The method as claimed in claim 8, wherein primers of the reaction mixture amplifies said region of the target nucleotide sequence by binding to a consensus sequence flanking the region having mutation or suspected of having mutation at Nth position.
12. The method as claimed in claim 8, wherein primers of the reaction mixture anneal at same location at 3' end of the consensus sequence and at different locations at 5' end of the consensus sequence.
13. The method as claimed in claim 8, wherein the amplification is carried out by technique selected from a group comprising Conventional Polymerase Chain Reaction, HotStart Polymerase Chain Reaction, Real Time Polymerase Chain Reaction and Isothermal Amplifications.
14. The methods as claimed in claims 7 and 8, wherein the mutation is selected from a group comprising unpredicted sequence variations, SNPs, deletions, alternate splice products, microsatellites and gene rearrangements or any combination thereof.
15. The primer set as claimed in claim 1 , the kit as claimed in claim 3 and the methods as claimed in claims 7 and 8, wherein the target nucleotide sequence is selected from a group comprising prokaryotic and eukaryotic genomic sequence or a combination thereof.
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