Mir-19a detection kit based on allglo probe fluorescence quantitative PCR and detection method thereof

A technology of mir-19a and detection kit, applied in the direction of DNA / RNA fragments, recombinant DNA technology, etc., can solve the problems of inaccurate detection of miRNA, low detection sensitivity and specificity, low specificity and sensitivity, and achieve cost Effect of low, weak background signal, high specificity and sensitivity

Inactive Publication Date: 2016-06-15
ZHONGSHAN HOSPITAL XIAMEN UNIV +1
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  • Abstract
  • Description
  • Claims
  • Application Information

AI Technical Summary

Problems solved by technology

Among them, northern blot technology is one of the early means of RNA detection, but its specificity and sensitivity are low. If the sample RNA content is low or there is degradation, it may not be detected; in situ hybridization technology is used to detect the distribution of miRNA at the tissue and cell level , while performing semi-quantitative detection of miRNA, its disadvantage is that it cannot accurately detect low-expression miRNA; microarray chip technology is a high-throughput detection technology that can simultaneously detect a large number of miRNAs in one or more samples , but there are problems such as time-consuming and labor-intensive chip fabrication, high labeling costs, and low detection sensitivity and specificity.
The reverse transcription primer based on the stem-loop structure can specifically recognize and amplify the mature miRNA sequence, but the precursor of the miRNA has not been amplified. The disadvantage of the Taqman-MGB probe for detecting miRNA is that the synthesis is expensive, which is not conducive to popularization.

Method used

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  • Mir-19a detection kit based on allglo probe fluorescence quantitative PCR and detection method thereof
  • Mir-19a detection kit based on allglo probe fluorescence quantitative PCR and detection method thereof
  • Mir-19a detection kit based on allglo probe fluorescence quantitative PCR and detection method thereof

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Embodiment 1

[0061] see figure 1 The embodiment of the miR-19a detection kit based on AllGlo probe fluorescent quantitative PCR of the present invention is provided with a box body 1, a partition 2, an exogenous reference bottle 3, a stem-loop reverse transcription reagent bottle 4, and a real-time fluorescent quantitative PCR Reagent bottle 5; partition 2 is set in box body 1, exogenous reference bottle 3, stem-loop reverse transcription reagent bottle 4, real-time fluorescent quantitative PCR reagent bottle 5 are inserted on partition 2, exogenous reference bottle 3 There is an exogenous reference, the stem-loop reverse transcription reagent bottle 4 is equipped with a stem-loop reverse transcription reagent, and the real-time fluorescent quantitative PCR reagent bottle 5 is equipped with a real-time fluorescent quantitative PCR reagent.

[0062] The exogenous reference can use cel-miR-39, etc., the cel-miR-39 is a class of nematode miRNA, its working concentration can be 5nmol, and its ...

Embodiment 2

[0066] Testing for plasma or serum miR-19a detection involves the following steps:

[0067] 1. Sample Collection

[0068] Collect heparin anticoagulated plasma or serum from 110 cases of esophageal cancer, 20 cases of leiomyoma, 18 cases of intraepithelial neoplasia, 14 cases of esophagitis, and 2 cases of esophageal polyps diagnosed by pathology, and put them in 1.5ml RNase-free EP tubes 400-500 μL was dispensed into each tube, and 200 μL was used for the next extraction, and the remaining plasma was frozen at -80°C.

[0069] 2. Extract microRNA

[0070] The miRNA extraction kit (DP501) produced by Tiangen Biotechnology Co., Ltd. was used to extract microRNA from samples (plasma or serum) according to the operating instructions. 200 μL of plasma or serum was added to an equal volume of lysate and allowed to stand for 5 minutes before adding exogenous Refer to cel-miR-395μL (working concentration is 5nmol / L), and then follow the instructions, and finally dissolve miRNA with ...

Embodiment 3

[0093] Example 3. Detection of tissue or cell miR-19a

[0094] 1. Sample handling:

[0095] a. Tissue: Grind the tissue in liquid nitrogen, add 1mL of lysate MZ (manufactured by Tiangen Biotechnology Co., Ltd.) for every 30-50mg of animal tissue or 100mg of plant tissue, and use a homogenizer for homogenization. It should exceed 10% of the MZ volume of the lysate.

[0096] b. Monolayer culture cells: directly add lysate MZ to the culture plate, every 10cm 2 Add 1mL LMZ to the area, and beat it several times with a sampler.

[0097] c. Cell suspension: centrifuge for 800r5min to take the cells, and discard the supernatant. Add 1mL Lysis Buffer MZ, shake with an oscillator or pipette several times to mix. Do not wash the cells before adding Lysis Buffer MZ to avoid RNA degradation.

[0098] 2. Tissue or cell miRNA extraction and enrichment

[0099] Use the miRNA extraction kit (DP501) produced by Tiangen Biotechnology Co., Ltd. to extract miRNA from tissues or cells accord...

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Abstract

miR-19a detection kit and detection method based on AllGlo probe fluorescent quantitative PCR. The detection kit is equipped with a box body, a partition, an exogenous reference bottle, a neck ring reverse transcription reagent bottle, and a real-time fluorescence quantitative PCR reagent bottle; the partition is set in the box body, and the exogenous reference bottle, neck ring reverse transcription reagent bottle , The real-time fluorescent quantitative PCR reagent bottle is inserted on the partition, the exogenous reference bottle is equipped with an exogenous reference, the neck ring reverse transcription reagent bottle is equipped with a neck ring reverse transcription reagent, and the real-time fluorescent quantitative PCR reagent bottle is equipped with a real-time fluorescent quantitative PCR reagents. Detection method: extract miRNA in the sample; use the stem-loop reverse transcription reagent provided by the detection kit to reverse miRNA into cDNA; use the real-time fluorescent quantitative PCR reagent provided by the detection kit to perform real-time fluorescent quantitative PCR amplification of cDNA; comprehensive analysis instrument Given the various data, set the threshold and baseline, and analyze the results.

Description

technical field [0001] The invention belongs to the fields of laboratory medicine, clinical medicine, biotechnology and molecular biology, and in particular relates to a miR-19a detection kit based on AllGlo probe fluorescence quantitative PCR and a detection method thereof. Background technique [0002] MicroRNA (miRNA) is a kind of non-coding RNA molecule of about 22 nucleotides widely present in eukaryotic cells, which participates in many physiological and pathological processes in organisms, by regulating gene expression, in cell proliferation, apoptosis , growth and development, cell differentiation, metabolism and other processes play an important role. The specific performance is that miRNA forms the initial primary transcript pri-miRNA to pre-miRNA in the nucleus, and then transports out of the nucleus, forms mature miRNA by shearing, and forms RISC (RNA-induced silencing complex) with Ago protein, etc. Partially inhibit or degrade the target mRNA sequence and part...

Claims

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Application Information

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Patent Type & Authority Applications(China)
IPC IPC(8): C12N15/11C12Q1/68
CPCC12Q1/6851C12Q1/6883C12Q1/6886
Inventor 林华月白永颖方宜臻张忠英
Owner ZHONGSHAN HOSPITAL XIAMEN UNIV
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