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Method for testing chromosome 22q11.2 microdeletion and microduplication

A micro-deletion and micro-duplication technology, applied in the field of bioengineering, can solve the problems of unsatisfactory positive rate, unavoidable false positive rate, uncertainty of results, etc. Effect

Inactive Publication Date: 2015-05-27
NANJING MATERNITY & CHILD HEALTH CARE HOSPITAL
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  • Abstract
  • Description
  • Claims
  • Application Information

AI Technical Summary

Problems solved by technology

However, as a semi-quantitative method, its false positive rate is inevitable
And its detection cost is high, it is difficult to promote on a large scale
[0005] The common disadvantage of the above methods for testing chromosome copy number changes is the uncertainty of the results
FISH technology is limited by the hybridization fragment of the probe, and the analysis of small deletions in chromosomal loci is prone to missed diagnosis. The judgment result of STRP analysis usually depends on the heterozygous band, and is affected by the heterozygosity of the target sequence and the analysis results of parental samples. Its positive rate is not completely satisfactory, and MLPA is a semi-quantitative method, its false positive rate is inevitable

Method used

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  • Method for testing chromosome 22q11.2 microdeletion and microduplication
  • Method for testing chromosome 22q11.2 microdeletion and microduplication
  • Method for testing chromosome 22q11.2 microdeletion and microduplication

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Experimental program
Comparison scheme
Effect test

Embodiment 1

[0048] Steps:

[0049] 1. Genomic DNA extraction: Resin TM Genomic DNA Extraction Kit (Shanghai Saibaisheng Technology Co., Ltd.); congenital heart disease patients and normal blood; Genomic DNA was extracted separately according to the requirements of the kit.

[0050] 2. Multiplex fluorescent quantitative PCR compound amplification

[0051] The complex amplification system includes 5 STR markers: D22S873, 22D_5_1, 22D_4_5, 22D_4_4, 22D_4_3 and an internal reference G6PDH;

[0052] The primer sequence is shown in the table below (FAM fluorescent label is added to the forward primer F of each STR site)

[0053]

[0054]

[0055] PCR amplification:

[0056] 25μl system includes: 35-80ng genomic DNA

[0057] 2.5μl 10×STR buffer (buffer) (promega)

[0058] 0.1 μM D22S873 primer

[0059] 0.2 μM 22D_5_1 primer

[0060] 0.4 μM 22D_4_5 primer

[0061] 1.1 μM 22D_4_4 primer

[0062] ...

Embodiment 2

[0085] Steps:

[0086] 1. Genomic DNA extraction: Resin-type TM Genomic DNA Extraction Kit (Shanghai Saibaisheng Technology Co., Ltd.); another congenital heart disease patient and normal blood; Genomic DNA was extracted separately according to the requirements of the kit.

[0087] 2. Multiplex fluorescent quantitative PCR compound amplification

[0088] The complex amplification system includes 5 STR markers: D22S873, 22D_5_1, 22D_4_5, 22D_4_4, 22D_4_3 and an internal reference G6PDH;

[0089] The primer sequence is shown in the table below (FAM fluorescent label is added to the forward primer F of each STR site)

[0090]

[0091]

[0092] PCR amplification:

[0093] 25μl system includes: 35-80ng genomic DNA

[0094] 2.5μl 10×STR buffer (promega)

[0095] 0.1 μM D22S873 primer

[0096] 0.2 μM 22D_5_1 primer

[0097] 0.4 μM 22D_4_5 primer

[0098] 1.1 μM 22D_4_4 primer

[0099] ...

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Abstract

The invention pertains to the filed of biological engineering and discloses a method for testing chromosome 22q11.2 microdeletion and microduplication; the testing method comprises the steps of: extracting genome DNA and conducting multiplex fluorescent quantitative PRC multiplex amplification; a multiplex amplification system comprises an internal reference G6PDH and 5 STR markers including D22S873, 22D_5_1, 22D_4_5, 2D_4_4 and 22 D_4_3; PCR amplified products are taken and modified to convert a double-chain product into a single-chain product on which a capilary electrophoretic analysis can be conducted; the capilary electrophoresis is adopted to analyze the length and yield of the modified product; and a quantity ratio analyzing method and / or a method of analyzing the position and quantity of peaks are adopted to judge whether the chromosome is normal and whether microdeletion or microduplication exists. The method can improve the testing reliability, shorten the testing time, lower the testing cost and be convenient for clinical use on large scale.

Description

technical field [0001] The invention belongs to the field of bioengineering and relates to a method for measuring micro-deletion and micro-duplication in chromosome 22q11.2 region. Background technique: [0002] The incidence rate of 22q11 microdeletion population is about 1 / 4000, and it is the most common genomic abnormality syndrome. The most common clinical manifestation is congenital heart defect (CHD). Other clinical manifestations include: facial deformity, immune deficiency, hypercalcemia , skeletal abnormalities, urinary system deformities, mild learning disabilities, etc. The most common CHDs are interrupted aortic arch, tetralogy of Fallot, ventricular septal defect, and persistent arterial trunk. Analysis of 22q11 microdeletion in CHD can not only explore the molecular mechanism of CHD, but also help in clinical diagnosis, genetic counseling and prenatal diagnosis. [0003] Although foreign countries have explored the relationship between 22q11 microdeletion and...

Claims

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Application Information

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Patent Type & Authority Patents(China)
IPC IPC(8): C12Q1/68
Inventor 许争峰易龙
Owner NANJING MATERNITY & CHILD HEALTH CARE HOSPITAL
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