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Digestion probe in PCR detection and kit thereof

A probe and target technology, applied in the field of biomedicine, can solve the problems of affecting detection sensitivity, high requirements for reaction conditions, and insufficient digestion efficiency

Pending Publication Date: 2022-02-18
BEIJING MICROREAD GENE TECH
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  • Summary
  • Abstract
  • Description
  • Claims
  • Application Information

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Problems solved by technology

Although the former is relatively simple to operate, it requires higher reaction conditions and it is difficult to detect multiple microsatellite sites at the same time.
The reaction conditions of the latter are relatively stable, and multiple sites can be detected at the same time, but because the digestion efficiency is not high enough, there are still a very large number of wild-type signals in the final detection results, which affects the detection sensitivity, especially in multiplex amplification. This detrimental effect is particularly pronounced in increasing
[0013] This phenomenon exists not only in microsatellite instability (MSI), but also in conventional PCR amplification, because in conventional detection, the base difference between the target fragment and other fragments is relatively large, and its impact on sensitivity is limited. However, if the fragments with other target fragments can be digested before amplification, the sensitivity will be greatly increased in the PCR amplification of target fragments

Method used

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  • Digestion probe in PCR detection and kit thereof
  • Digestion probe in PCR detection and kit thereof
  • Digestion probe in PCR detection and kit thereof

Examples

Experimental program
Comparison scheme
Effect test

Embodiment 1

[0090] Example 1: Conventional MSI detection.

[0091] Conventional MSI detection requires simultaneous detection of two samples from the same individual, usually using tumor tissue samples as test samples, and peripheral blood or paracancerous tissue samples as control samples. By comparing the results of tumor tissue samples with those of control samples, it is determined whether there is MSI in the sample.

[0092] The sample tested in this example comes from a rectal cancer patient. The control sample was the peripheral blood sample A collected before operation, and the test sample was the paraffin-embedded tumor tissue sample B.

[0093] 1.1 DNA extraction

[0094] Use a routine blood extraction kit to extract DNA from peripheral blood sample A; use a conventional paraffin-embedded tissue DNA extraction kit to extract DNA from tumor tissue sample B. ul.

[0095] 1.2 PCR amplification

[0096] Use the microsatellite instability detection kit (patent CN201810126825.6) ...

Embodiment 2

[0131] Example 2: Detection of digested MSI

[0132] Adding a step of digestion before the conventional MSI detection amplification can specifically digest the wild-type DNA fragments, thereby increasing the abundance of microsatellite unstable DNA fragments, and ultimately improving the sensitivity of MSI detection.

[0133] A non-optimized common digestion probe was used in this implementation. The tested sample is the same sample as the control sample in Example 1, the peripheral blood sample A collected before the operation.

[0134] 2.1 cfDNA extraction

[0135] Plasma was separated from peripheral blood A (centrifuged at 1600 rcf for 10 min; centrifuged at 16000 rcf for 10 min). Use the cfDNA extraction kit to extract the cfDNA in the plasma of peripheral blood sample A, measure the concentration with a UV spectrophotometer after the extraction, and dilute to 10ng / ul.

[0136] 2.2 Probe digestion

[0137]The probes used were derived from reference 2 (Ladas I, Yu F, L...

Embodiment 3

[0163] Example 3: MSI detection using optimized digestion probe digestion

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Abstract

The invention relates to a digestion probe in PCR (Polymerase Chain Reaction) detection and a kit thereof. The digestion probe, has a structure of digestion probe 5' end-probe middle part-probe 3' end. By adjusting the digestion probe structure and introducing basic group modification, so that the binding capacity of the 5' end of the digestion probe is relatively weak, and the binding capacity of the 3' end of the digestion probe is relatively strong, therefore, on the premise of ensuring the digestion efficiency of a digestion target fragment, the digestion specificity is enhanced, detection signals corresponding to the target fragment are enriched more effectively, finally, the detection sensitivity is greatly improved, and liquid biopsy can be achieved.

Description

technical field [0001] The invention belongs to the detection technology of clinical molecular diagnosis in the field of biomedicine. The invention relates to a digestion probe and a kit in PCR detection, in particular to a wild-type target fragment digestion probe and its application in the detection of microsatellite instability, which can improve the detection sensitivity of microsatellite instability (MSI), especially can be applied MSI detection method for liquid biopsy. Background technique [0002] Microsatellite sequence refers to a short tandem repeat structure with a core sequence of 1 to 6 bases, and these repeat sequences are distributed throughout the human genome. The phenomenon of microsatellite sequence length change caused by insertion or deletion mutations during DNA replication is called microsatellite instability (Microsatellite Instability, MSI). [0003] Microsatellite instability (MSI) phenomenon exists in many solid tumors. The tumor types with the...

Claims

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Application Information

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Patent Type & Authority Applications(China)
IPC IPC(8): C12Q1/686C12N15/11
CPCC12Q1/686C12Q2525/151
Inventor 陈莹张奇张颖张晔
Owner BEIJING MICROREAD GENE TECH
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