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Primer combinations, methods and kits for constructing multiple hemophilia targeting libraries based on high-throughput sequencing

A primer combination and construction method technology, applied in biochemical equipment and methods, combinatorial chemistry, chemical library, etc., can solve the problems of gene coverage, random missed detection, cumbersome operation, etc., to avoid workload and economic costs, save The effect of time cost and simple operation

Active Publication Date: 2020-07-17
THE FIRST AFFILIATED HOSPITAL OF ARMY MEDICAL UNIV
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  • Summary
  • Abstract
  • Description
  • Claims
  • Application Information

AI Technical Summary

Problems solved by technology

Therefore, the heterogeneity and individual differences of gene mutations determine that the gene mutation detection of hemophilia and congenital hemorrhagic disease needs to cover all exons and intron splicing regions of the disease-causing gene in order to be accurate and comprehensive. Covering and identifying its pathogenic mutations without omission, simply detecting a few hot mutation sites of a gene will result in a large number of missed detections
At present, there is no genetic testing kit for simultaneous detection and identification of multiple hemophilias in the market.
[0009] At present, IS-PCR is used to detect F8 gene inversion, and Sanger sequencing is used to detect single hemophilia point mutations and indels. This method can only detect certain hotspot mutations of a single gene at a time, and it is difficult to detect Potential disease-causing sites and new mutation sites of the entire gene are all detected, and more than 60% of false negatives may occur. Differential diagnosis needs to be detected one by one gene by one site, and the operation is cumbersome, time-consuming and labor-intensive
With the advancement of technology, whole-exome high-throughput sequencing has realized the simultaneous detection of multiple gene variations, but whole-exome high-throughput sequencing is expensive, and it is very wasteful to detect a small number of single-gene diseases. Due to the huge size of the human genome and the limitations of the whole exome sequencing technology itself, there will be a small number of genes that cannot be covered and randomly missed

Method used

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  • Primer combinations, methods and kits for constructing multiple hemophilia targeting libraries based on high-throughput sequencing
  • Primer combinations, methods and kits for constructing multiple hemophilia targeting libraries based on high-throughput sequencing
  • Primer combinations, methods and kits for constructing multiple hemophilia targeting libraries based on high-throughput sequencing

Examples

Experimental program
Comparison scheme
Effect test

Embodiment 1

[0024] Example 1 Primer combination

[0025] A total of 128 target regions were targeted at all exons, splicing regions, partial promoter regions and intron regions of 7 genes including F8, F9, F11, vWF, F2, F7 and SRY. Among them, the F8 and F9 genes also include the promoter region, the F2 gene also includes a part of the 3'UTR region, and the F8 gene also includes a part of intron 4. A total of 225 pairs of primers were designed and synthesized, and their base sequences are shown in SEQID No. 1~shown in SEQ ID No.450.

[0026] The detected genes and coverage areas are as follows:

[0027]

[0028] The optimized primers are as follows:

[0029]

[0030]

[0031]

[0032] Send the above-mentioned SEQ ID No.1 to SEQ ID No.450 to Biological Company for synthesis, and mix all or part of the primer pairs of SEQ ID No.1 to SEQ ID No.450 in equal amounts, and load them in the same packaging tube or at most 2 packages In the tube, a pool of primers is formed, which ca...

Embodiment 2

[0033] Example 2 Detection sample processing and DNA extraction

[0034] The detection sample of the present invention may be whole blood, blood clot, fresh pathological tissue, paraffin-embedded tissue, and this embodiment only uses whole blood sample as an example for illustration.

[0035] In order to reduce the interference of various anticoagulants on the PCR reaction, venous blood should be collected with EDTA-K2 anticoagulant blood collection tubes. The venous blood should be extracted and purified every day. If it cannot be extracted in time on the same day, it should be stored in a 4°C refrigerator. save. Conventional DNA extraction and purification methods such as DNA extraction kits or automatic DNA extractors can be used. The DNA concentration was detected with a Nanodrop 2000 trace nucleic acid and protein detector, and the 260 / 280 ratio and 260 / 230 ratio were determined. The extracted DNA is subjected to 0.5% agarose gel electrophoresis, and a clear electrophor...

Embodiment 3

[0036] Example 3 Constructing Multiple Hemophilia Targeting Libraries

[0037] Standardize the sample DNA extracted in Example 2, adjust the concentration to 40-50ng / ul as the amplification template, and use all or part of the primers from SEQ ID No.1 to SEQ ID No.450 described in Example 1 The primer mixture pool composed of primers is used for ultra-high multiplex PCR amplification. Perform PCR amplification according to the following amplification system and conditions, and perform ultra-high multiplex PCR amplification according to the multiple ratio volume or equal concentration system of the following system:

[0038]

[0039] Preferably, the amplification conditions are: 95°C for 10 min; 98°C for 15 s, 60°C for 5 min, 9-11 cycles; 10°C ∞.

[0040] The amplification product is purified by magnetic beads, non-specific products are removed, and then purified to obtain a targeted library of the target gene. High-throughput sequencing primers and barcode tags can be add...

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Abstract

The invention discloses a primer combination, a method and a kit for constructing multiple hemophilia targeting libraries based on high-throughput sequencing. The base sequence of the primer group ofthe present invention is SEQ ID No. 1 to SEQ ID No. 450, Overridden F8, F9, F11, vWF, F2, F7 and SRY are all exons of 7 genes, The splicing region, partial promoter region and intron region, 128 target regions and 225 pairs of primers were used to detect gene mutations in hemophilia A, hemophilia B, hemophilia C, von Willebrand disease, factor II deficiency and factor VII deficiency simultaneously. The invention can be applied to detection and screening of pathogenic sites of congenital hemorrhagic diseases such as hemophilia, screening of family members and scientific research on corresponding pathogenic mutations. The method is simple, accurate and time-consuming, and greatly saves the time cost and labor cost of Sanger sequencing gene by gene segment by segment detection.

Description

technical field [0001] The invention relates to the field of biotechnology, in particular to a primer combination, a method and a kit for constructing various hemophilia targeting libraries based on high-throughput sequencing. Background technique [0002] Hemophilia is a group of congenital bleeding disorders with hereditary coagulation dysfunction. Its common features are the deficiency of certain coagulation factors, the generation of active thromboplastin, prolonged coagulation time, and a lifelong tendency to bleeding after minor trauma. Severe patients "Spontaneous" bleeding can occur without obvious trauma. On May 11, 2018, five departments including the National Health Commission jointly formulated the "First Batch of Rare Disease List", and hemophilia was included in it. Large-scale epidemiological surveys show that the incidence of hemophilia is 15-20 / 100,000, and it is the most common disease among congenital bleeding disorders. According to literature reports, ...

Claims

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Application Information

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Patent Type & Authority Patents(China)
IPC IPC(8): C12Q1/6869C40B50/06C12N15/11
CPCC12Q1/6869C40B50/06C12Q2535/122
Inventor 谭文婷邓国宏但芸婕孙凤明
Owner THE FIRST AFFILIATED HOSPITAL OF ARMY MEDICAL UNIV
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