CN1281901A - Homogeneous pluorescence probe PCR mycobacterium tuberculosis detection method - Google Patents

Homogeneous pluorescence probe PCR mycobacterium tuberculosis detection method Download PDF

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CN1281901A
CN1281901A CN 99112336 CN99112336A CN1281901A CN 1281901 A CN1281901 A CN 1281901A CN 99112336 CN99112336 CN 99112336 CN 99112336 A CN99112336 A CN 99112336A CN 1281901 A CN1281901 A CN 1281901A
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pluorescence
homogeneous
pcr
mycobacterium tuberculosis
probe
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CN1127575C (en
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李庆阁
梁基选
栾国彦
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XIAMEN TAILUN BIO-ENGINEERING Co Ltd
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XIAMEN TAILUN BIO-ENGINEERING Co Ltd
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Abstract

Ac cording to tubercle bacillus (TB) gene sequence said invention adopts TB chromosome insertion sequence IS 986 contrived synthetic primer, uses polymerase chain reaction (PCR) to implement amplification of TB specific fragment and uses the hybridization of molecular beacon probe and amplification product as method for determination of result, and utilizes the fluorimeter to directly measure the fluorescent intensity of reaction tube to detect that said specimen has tubercle bacillus or not.

Description

Homogeneous pluorescence probe PCR mycobacterium tuberculosis detection method
The present invention relates to the detection method of a kind of PCR tubercule bacillus.
Polymerase chain reaction (PCR) is the technology of a kind of amplification in vitro dna fragmentation of growing up in the later stage eighties, can obtain millions of specific DNA sequences copies in a few hours.Theoretically, PCR can reach 1 tubercule bacillus in conjunction with the sensitivity of electrophoresis detection, but exist in the clinical samples amplified reaction is had inhibiting factor, the sensitivity that PCR is detected reduces, in addition because the high sensitivity of PCR reaction, the pollution of amplified production is easy to generate false positive again, and false positive and false negative cause sensitivity that PCR detects and specificity and theoretic gap bigger.
The objective of the invention is to adopt nucleic acid amplification reaction bonding probes hybridization technique to improve sensitivity and specificity that PCR detects.
The present invention is according to tubercule bacillus (TB) gene order, the design synthetic primer, (PCR) increases to the TB specific fragment with the polymerase chain reaction, use the hybridization of molecular beacon probe and amplified production, method for measuring as a result of, directly measure the fluorescence intensity of reaction tubes by photofluorometer, detect sample and whether have tubercule bacillus.Molecular beacon probe is a kind of hair clip type oligonucleotide probe based on the design of fluorescence energy transfer phenomenon, be loop-stem structure on the space structure, the ring sequence is and target nucleic acid complementary probe, the stem sequence is by constituting with the irrelevant complementary sequence of target sequence, and an end of stem connects fluorescence molecule, and the other end connects quencher molecule, during no target sequence, the space structure of molecular beacon is constant, and fluorescence molecule and quencher molecule are very approaching, and this moment, fluorescence was by cancellation; When target sequence was arranged, the ring sequence of molecular beacon can combine with the target sequence specificity, and loop-stem structure is opened, and fluorescence molecule separates with quencher molecule, and this moment, fluorescence molecule just can send fluorescence, and the fluorescence that sends just can detect by fluor tester.Its main process is as follows:
According to the PCR reaction principle, select suitable Taq enzyme, starting material such as dNTP, synthetic Auele Specific Primer in addition, adds molecular beacon probe, is mixed with the PCR reaction system.And with sample extracting solution (tri-distilled water preparation, include 2%TritonX-100,1%NP-40 and 0.04M Sodium octoate) carry out clinical sample and extract, then, carry out pcr amplification, pass through the yin and yang attribute of the change judgement sample of measurement reaction solution fluorescence intensity after reaction is finished.
The TB probe: the oligonucleotide probe of design and target complement sequence in two primer amplification fragments, 5 ' end is modified with EAM, and 3 ' end is with amido modified.EAM-5 '-GCG AGG AAC GGC TGA TGA CCA AAC TCT CGC-3 ' DABCYL (the line part is the hair clip shank, and uncrossed part is and target sequence specificity complementary sequence)
Its space structure is as follows:
Figure 9911233600051
The present invention utilizes molecular beacon probe, after pcr amplification is finished on pocket luminoscope direct reading, judge yin and yang attribute.The molecular beacon two ends indicate fluorescent agent and quencher respectively, the generation fluorescent energy transmits, according to the Forster theory, 6 powers of distance are inversely proportional between fluorescence energy transfer efficient and the fluorescent substance-quencher, molecular beacon at the hair clip state because fluorescent agent and quencher are extremely close, the transfer efficiency of fluorescence almost is 100%, thereby fluorescence is almost completely by cancellation.And the distance increase owing to fluorescent agent and quencher is very big when launching, and the fluorescence of fluorescent agent is 100% recovery almost.So the signal/background of this reagent is higher than very, so sensitivity is very high.Molecular beacon needs at first consumed energy expansion hair clip handle with combining of target sequence in addition, even if hairpin loop and target sequence can not mate the difference of a base fully, the energy that discharges in conjunction with the back does not also support the energy that launches the consumption of hair clip handle, thereby crossover process finally can't be finished.The setting of hair clip handle energy barrier obviously improves the hybridization specificity of " molecular beacon ".Add with pocket luminoscope simple to operately, be suitable for Clinical Laboratory and use.
The embodiment of the invention is as follows:
The present invention is formulated as follows test kit: its raw material is selected for use as follows:
The TB primer: with reference to designing synthetic primer with TB insertion sequence IS986, this primer tool group specificity is given birth to worker bio-engineering corporation by Shanghai and is synthesized.INS-1:5 '-CGT GAG GGC ATC GAG GTG GC-3 ' INS-2:5 '-GCG TAG GCG TCG GTG ACA AA-3 ' TB probe: the oligonucleotide probe of design and target complement sequence in two primer amplification fragments, 5 ' end is modified with FAM, 3 ' end is given birth to worker bio-engineering corporation by Shanghai and is synthesized with amido modified.
FAM-5′-GCG?AGG?AAC?GGC?TGA?TGA?CCA?AAC?TCT?CGC-3′-NH 2
The Taq enzyme: Shanghai Promega company, concentration: 5U/ μ l, attached Taq storage buffer (50% glycerine, 20mM Tris-HCl (pH8.0), 100mM KCl, 0.1mM EDTA, 1mM DTT,
0.5%Tween-20,0.5%N?P-40)。DNTP (dATP, dTTP, dCTP, dGTP): available from Pharmacia company, concentration 100mM.
Sample source: positive: bacille Calmette-Guerin vaccine and positive clinical samples that the Shanghai institute of Biological Products is produced,
Identify institute's tubercule bacillus liquid available from biological products.Negative sample: collect healthy people's sputum etc.
PCR thin-walled reaction tubes: available from U.S. PE company, specification 0.5ml.Chemical reagent:
DABCYL-SE: U.S. Molecular Probes.
Fluorescein reference liquid: U.S. Bio-Rad, 1mM DMSO solution.
NP-40: U.S. AMRESCO.
TritonX-100: U.S. AMRESCO.
Tris: U.S. AMRESCO.
Paraffin oil: Sigma.
Sodium octoate: Sigma.
Other chemical reagent is homemade analytical pure.
Manufacturing course
The mark of TB molecular beacon probe and purifying
According to the resultant quantity that manufacturer provides, dispose the NaHCO of 100 μ M probes 3-Na 2CO 3Solution (0.1M, pH9.0) 50 μ l, to the N that wherein slowly adds 10 μ l 200mg/ml DABCYL-SE, N-dimethylformamide solution, stirring reaction spends the night.Centrifugal removal precipitation, solution is crossed G-25 post (0.1M acetic acid triethylamine, pH6.5 pre-equilibration) and is removed free dye.Press chromatogram (Bio-Rad) purifying, linear elution, 20%-70% solution B (0.1M acetic acid triethylamine: CH in the last C-18 reversed-phase column (Waters) 3CN=25: 75 (V/V), pH6.5); Solution A: 0.1M acetic acid triethylamine, pH6.5; Flow velocity 1ml/min; Time 20min.Detect with the 260nm wavelength, collect main peak.Use Nanosep 3K (Gelman) ultrafiltration and concentration at last, be dissolved in (10mM Tris-HCl pH8.3,1.5mMMgCl in the 100 μ l damping fluids 2), quantitative with ultraviolet spectrophotometer.Transferring concentration is 100 μ M ,-20 ℃ of storages.
The preparation of PCR reaction mixture
The preparation of 10 * PCR damping fluid
100mM?Tris-HCl(pH8.3)
500mM?KCl
20mM?MgCl 2
1% TritonX-100
With tri-distilled water preparation, autoclaving, sealing ,-20 ℃ of storages.
The dissolving of TB primer and mensuration
According to the synthetic OD value that manufacturer provides, with the tri-distilled water dissolving, with UV spectrophotometer measuring primer content, regulating and guiding substrate concentration is 100 μ M.
The PCR reaction mixture: 10 * PCR damping fluid includes TB two and draws with 8 times of dilutions of aseptic tri-distilled water
Each 0.5 μ M of thing, probe 0.25 μ M, dNTP 250 μ M.
The packing of PCR reaction mixture: aseptic subpackaged in the 0.5ml centrifuge tube, every 0.45ml.
Contain the preparation of enzyme reaction pipe
Taq enzyme preparation: become 1U/ μ l with Taq enzyme storage buffer dilution Taq enzyme.
Be sub-packed in the 0.5ml PCR thin-walled tube, every pipe 1.2 μ l add 50 μ l Valelinum Liquidums.
Sample extracting solution
Preparation: the tri-distilled water preparation includes 2%TritonX-100,1%NP-40 and 0.04M Sodium octoate.
Packing: divide behind the autoclaving to be filled in the 1.5ml centrifuge tube every pipe volume 1.2ml.
The yin and yang attribute contrast
Negative control preparation: healthy people's sputum is diluted in 0.9% physiological saline at 1: 20 after trysinization.
Positive control preparation: negative control dilution tubercule bacillus that biopsy provides, content 10 3Individual bacterium/ml.
Packing: aseptic subpackaged in the 0.5ml centrifuge tube, every 0.5ml.
Zeroing pipe and correction pipe;
The packing of zeroing pipe: Taq enzyme store buffer liquid (not containing the Taq enzyme) is sub-packed in the 0.5ml PCR thin-walled tube, and every pipe 1.2 μ l add 50 μ l Valelinum Liquidums.
Proofread and correct the pipe packing: the standard fluorescence cellulose solution that contains 30nM is sub-packed in the 0.5ml PCR thin-walled tube, every pipe 50 μ l.
Detect step:
(1) sputum sample process:
1 adds the 4%NaOH of 2 times of volumes in sputum, jolting was repeatedly put room temperature 20 minutes, made it abundant liquefaction.
2 get 0.5ml liquefaction sputum adds in the 0.5ml centrifuge tube, in centrifugal 10 minutes of 1.4 ten thousand rev/mins of high speed tabletop centrifuges, abandons supernatant liquor.
3 add sterile purified water 0.5ml in the precipitation in, the vibration mixing, 1.4 ten thousand rev/mins centrifugal 10 minutes, abandon supernatant liquor.
4 repeating steps (3).
5 add sample extracting solution 50 μ l in precipitation, behind the vibration mixing, put in 100 ℃ of water-baths 15 minutes, and after the taking-up, centrifugal 5 minutes of 1.5 ten thousand rev/mins of sample hoses, supernatant liquor promptly can be used as reaction template.
6 positive controls and negative control do not need with NaOH liquefaction, direct 1.4 ten thousand rev/mins centrifugal 10 minutes, abandon supernatant liquor.Carry out the 5th the step get final product.
(2) pcr amplification reaction:
Taking-up contains the enzyme reaction pipe and adds 20 μ l reaction mixtures, add the sample supernatant (directly adding 20 μ l reaction mixtures and 4 μ l sample extracting solutions in the zeroing pipe) that 4 μ l have handled again, mixing (is noted: can not high vibration, avoid producing too much foam) after, 10,000 rev/mins centrifugal 20 seconds, can circulate by pcr amplification instrument on the following program.
(3) result judges:
1. instrument calibration:
The pipe that will return to zero is earlier put into TD-360 type luminoscope and is returned to zero, and will proofread and correct pipe again and put into luminoscope, and proofreading and correct reading is 1000.
2. sample determination:
The reaction tubes that will take out from the pcr amplification instrument is put into the luminoscope reading one by one.
3. the result judges: positive fluorescent intensity/negative control fluorescence intensity<2.0 are negative in fluorescent intensity/negative control fluorescence intensity 〉=2.0
(annotate: negative control fluorescence intensity<50 o'clock, by 50)
The present invention utilizes molecular beacon probe, after pcr amplification is finished on pocket luminoscope direct reading, judge yin and yang attribute.Not only eliminated the pollution of amplified production, simplified operation,, guaranteed specificity and the sensitivity measured, and might develop into quantitative assay more owing to the existence of unique molecular beacon probe.Add with pocket luminoscope simple to operately, be suitable for Clinical Laboratory and use.

Claims (9)

1. homogeneous pluorescence probe PCR mycobacterium tuberculosis detection method, its feature adopt PCR method amplification tubercule bacillus (TB) gene order, utilize the hybridization of molecular beacon and amplified production, and the fluorescence intensity of measurement reaction solution, carry out mensuration as a result.
2. according to the homogeneous pluorescence probe PCR mycobacterium tuberculosis detection method of claim 1, it is characterized in that selecting the TB primer to be: a pair of primer of tubercule bacillus insertion sequence IS986: ISN-1:5 '-CGT GAG GGC ATC GAG GTG GC-3 ' INS-2:5 '-GCG TAG GCG TCG GTG ACA AA-3 '.
3. according to the homogeneous pluorescence probe PCR mycobacterium tuberculosis detection method of claim 1, it is characterized in that its TB probe: the oligonucleotide probe of design and target complement sequence in two primer amplification fragments, 5 ' end is modified with FAM, 3 ' end is with amido modified, and its sequence of mark DABCYL is: FAM-5 ,-GCG AGG AAC GGC TGA TGA CCA AAC TCT CGC-3 ' DABCYL.
4. according to the homogeneous pluorescence probe PCR mycobacterium tuberculosis detection method of claim 1, it is characterized in that the homogeneous pluorescence probe PCR mycobacterium tuberculosis detection kit comprises: contain the enzyme reaction pipe; Reaction mixture; Positive control; Negative control; Sample extracting solution; The zeroing pipe; Proofread and correct pipe; Working instructions.
5. according to the homogeneous pluorescence probe PCR mycobacterium tuberculosis detection method of claim 1, it is characterized in that homogeneous pluorescence probe PCR mycobacterium tuberculosis detection kit reaction mixture is: 10 * PCR damping fluid (100mMTris-HCl pH8.3; 500mM KCl; 20mM MgCl 21%TritonX-100) with 8 times of dilutions of aseptic tri-distilled water, include each 0.5 μ M of TB two primers, probe 0.25 μ M, dNTP 250 μ M.
6. according to the homogeneous pluorescence probe PCR mycobacterium tuberculosis detection method of claim 1, it is characterized in that the homogeneous pluorescence probe PCR mycobacterium tuberculosis detection kit contains the enzyme reaction pipe and is: become 1U/ μ l with Taq enzyme storage buffer dilution Taq enzyme.Be sub-packed in the 0.5ml PCR thin-walled tube, every pipe 1.2 μ l add 50 μ l Valelinum Liquidums.
7. according to the homogeneous pluorescence probe PCR mycobacterium tuberculosis detection method of claim 1, it is characterized in that homogeneous pluorescence probe PCR mycobacterium tuberculosis detection kit zeroing pipe is: Taq enzyme store buffer liquid (not containing the Taq enzyme) is sub-packed in the 0.5ml PCR thin-walled tube, every pipe 1.2 μ l add 50 μ l Valelinum Liquidums.
8. according to the homogeneous pluorescence probe PCR mycobacterium tuberculosis detection method of claim 1, it is characterized in that sample extracting solution is: the tri-distilled water preparation includes 2%TritonX-100,1%NP-40 and 0.04M Sodium octoate.
9. according to the homogeneous pluorescence probe PCR mycobacterium tuberculosis detection method of claim 1, it is characterized in that the preparation process of molecular beacon is as follows: the NaHCO that gets the 100mM probe 3-Na 2CO 3Solution 50 μ L, to the N that wherein slowly adds 10uL200mg/ml DABCYL-SE, N-dimethylformamide solution, stirring reaction is crossed liquid.Centrifugal removal precipitation, solution is crossed G-25 post (0.1M acetic acid triethylamine, pH6.5 pre-equilibration) and is removed free dye.Press chromatogram (Bio-Rad) purifying, linear elution, 20-70% solution B (0.1M acetic acid triethylamine: CH in the last C-18 reversed-phase column (Waters) 3CN=25: 75 (V/V), pH6.5).Solution A: 0.1M acetic acid triethylamine, pH6.5: flow velocity 1mL/min: time 20min.Detect with the 260nm wavelength, collect main peak, use Nanosep3K (Gelman) ultrafiltration and concentration at last.
CN 99112336 1999-07-22 1999-07-22 Homogeneous pluorescence probe PCR mycobacterium tuberculosis detection method Expired - Fee Related CN1127575C (en)

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Cited By (3)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN100427927C (en) * 2005-12-08 2008-10-22 中国农业科学院作物科学研究所 Green smut bug real-time fluorescent quantitative PCR test kit and its use
CN101560542B (en) * 2008-04-14 2013-12-18 福建医科大学 Diagnostic kit for mcirocolony molecular beacon culturing mycobacterium tuberculosis, preparation method and application
CN106226273A (en) * 2016-07-05 2016-12-14 无锡市第二人民医院 A kind of method for quick of microRNA

Families Citing this family (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN101050475B (en) * 2007-04-25 2010-05-26 中国人民解放军第三军医大学第一附属医院 Method for constructing DNA probe in shape of asymmetric ring type hair clip, and application

Cited By (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN100427927C (en) * 2005-12-08 2008-10-22 中国农业科学院作物科学研究所 Green smut bug real-time fluorescent quantitative PCR test kit and its use
CN101560542B (en) * 2008-04-14 2013-12-18 福建医科大学 Diagnostic kit for mcirocolony molecular beacon culturing mycobacterium tuberculosis, preparation method and application
CN106226273A (en) * 2016-07-05 2016-12-14 无锡市第二人民医院 A kind of method for quick of microRNA
CN106226273B (en) * 2016-07-05 2018-09-25 无锡市第二人民医院 A kind of rapid detection method of microRNA

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