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Multiple real-time fluorescent PCR detection kit for Y chromosome microdeletion

A detection kit and technology for Y chromosome, which is applied in the field of multiple real-time fluorescent PCR detection kits for male Y chromosome microdeletion, which can solve the problems of non-sequence specificity of dyes, reduced throughput, and low throughput, so as to avoid false negatives and false positive results, increase throughput, and increase amplification efficiency

Active Publication Date: 2012-10-03
郭奇伟
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  • Abstract
  • Description
  • Claims
  • Application Information

AI Technical Summary

Problems solved by technology

However, due to the non-sequence specificity of the dye, only singleplex PCR can be performed, which not only reduces the throughput, but also must rely on melting curve analysis to distinguish target fragments from primer-dimers
The current probe method is also single-plex PCR, which not only reduces the throughput, but also easily causes false positive results because there is no internal reference

Method used

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  • Multiple real-time fluorescent PCR detection kit for Y chromosome microdeletion
  • Multiple real-time fluorescent PCR detection kit for Y chromosome microdeletion
  • Multiple real-time fluorescent PCR detection kit for Y chromosome microdeletion

Examples

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Embodiment 1

[0045] Example 1 Multiplex real-time fluorescent PCR for simultaneous detection of 6 AZF deletion sites in two tubes

[0046] 1. Materials

[0047] 1. Instrument:

[0048] Real-time PCR instrument, pipette, centrifuge.

[0049] 2. Primer design:

[0050] In the present invention, 8 pairs of homologous tailing primers and one universal primer are designed for the detection of 6 microdeletion sites of the Y chromosome, and 8 hydrolysis probes are designed in this example to detect the corresponding target fragments. In this example, the reaction is carried out in two reaction tubes, A and B. The sequences of primers and probes used in the A tube reaction are shown in Table 1, and the sequences of the primers and probes used in the B tube reaction are shown in Table 2

[0051] Table 1A Tube Primer and Probe List

[0052]

[0053]

[0054] Table 2B Tube Primer and Probe List

[0055]

[0056] 3. Reagents

[0057] 1×PCR buffer: 10mmol / L Tris-HCl (pH 8.3), 50mmol / L K...

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Abstract

The invention relates to the chromosome deletion detection field, and especially relates to a multiple real-time fluorescent PCR detection kit for Y chromosome microdeletion. The kit detects gene deletion at sY84 and sY86 loci of a Y chromosome AZFa subregion, sY127 and sY134 loci of a Y chromosome AZFb subregion, and sY254 and sY255 loci of a Y chromosome AZFc subregion by real-time fluorescent PCR. The kit realizes a stable and high-efficient multiple PCR reaction system by using homologous tailed primers and universal primers, adopts nucleic acid probes labeled by different fluorescent genes to indicate the presence of target fragments, and thus realizes the fastest simultaneous detection of sequences on 6 AZF deletion hotspots and 2 internally controlled genes by two tubes. The kit of the invention can be used for detection of male Y chromosome microdeletion genes, and has the advantages of high speed, accuracy, high throughput, low cost, no pollution, and the like.

Description

technical field [0001] The invention relates to the field of chromosome deletion detection, in particular to a multiple real-time fluorescent PCR detection kit and detection method for male Y chromosome microdeletion. Background technique [0002] Worldwide, about 15% of couples of childbearing age suffer from infertility, of which male factors account for about 50%. Studies have shown that more than 35% are due to genetic factors, mainly Klinefelter syndrome and Y chromosome microdeletion. At present, it is known that there is azoospermia factor (AZF) on the Y chromosome, which is closely related to the production of sperm. There are three AZF subregions on the long arm of the Y chromosome—AZFa region, AZFb region, and AZFc region. Genetic microdeletions in these regions can cause spermatogenesis disorders, oligospermia, weak spermatozoa, and even azoospermia, leading to male infertility. [0003] In recent years, assisted reproductive technology has developed rapidly, a...

Claims

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Application Information

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Patent Type & Authority Applications(China)
IPC IPC(8): C12Q1/68
Inventor 郭奇伟周裕林江雨左正宏
Owner 郭奇伟
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