Fast and efficient construction method of normalized full-length cDNA library

A library construction, full-length technology, applied in the field of modern molecular biology, can solve the problems of high cost, low efficiency, unfavorable gene cloning of large fragments, etc., and achieve the effect of small requirements

Active Publication Date: 2012-11-28
BEIJING VJT BIO CO LTD
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Problems solved by technology

[0017] Existing methods for constructing full-length cDNA libraries have their own characteristics and have certain defects. Some of them involve PCR amplification, which can easily change the representativeness of clones in the library and affect the cloning of difficult-to-amplify genes; Plasmids are carriers, which are not conducive to the cloning of large fragments of genes;

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  • Fast and efficient construction method of normalized full-length cDNA library
  • Fast and efficient construction method of normalized full-length cDNA library
  • Fast and efficient construction method of normalized full-length cDNA library

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[0051] The preferred embodiments of the present invention will be described in detail below in conjunction with the accompanying drawings; it should be understood that the preferred embodiments are only for illustrating the present invention, rather than limiting the protection scope of the present invention.

[0052] The process of constructing cDNA library in the present invention can be divided into three parts: 1) mRNA subtraction / homogenization processing; 2) full-length cDNA acquisition; 3) second-strand cDNA synthesis and library acquisition. In these three parts, the subtraction / normalization process adopts the method of directly synthesizing the first strand of cDNA on the magnetic beads and hybridizing with the mRNA, then using the magnetic bead separation method to remove the highly expressed mRNA, and finally obtain the rare expressed mRNA; The methods and steps of the other two parts combine the improved Oligo-capping method to obtain full-length mRNA in one step a...

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Abstract

The invention relates to a fast and efficient construction method of a normalized full-length cDNA library. The method consists of: using specific 5-OH oligonucleotide to close non-full-length mRNA, then employing tobacco acid pyrophosphatase to remove a cap structure from the mRNA5' end to make a phosphate group at the cap structure of the mRNA5' end exposed, adopting an efficient RNA connection system to connect a section of optimized oligomeric RNA to the mRNA 5' end to serve as a primer binding site for triggering synthesis of second strand cDNA, finally conducting reverse transcription, two-strand synthesis as well as graded purification, and cloning the double-stranded DNA into a vector. The method can concisely and efficiently screen full-length mRNA, and realizes full-length mRNA capture of eukaryotes. The mRNA5' tail end contains a biotin label, which can be used for full-length mRNA separation. The used oligonucleotide primer contains optimized modification method and a nucleotide sequence, thus being able to realize full-length mRNA capture of eukaryotes, reverse transcription and DNA synthesis.

Description

technical field [0001] The invention relates to a fast and efficient method for constructing a uniform full-length cDNA library, which belongs to the technical field of modern molecular biology. Background technique [0002] The full-length cDNA library can not only greatly improve the process of gene sequencing and bioinformatics analysis, but also facilitates later protein expression and functional analysis. For organisms that cannot carry out whole genome sequencing, it is an important way to conduct functional genome research. Even after the complete genome sequencing of model organisms, such as Arabidopsis thaliana, rice, and Caenorhabditis elegans, molecular biologists still constructed full-length cDNA libraries of the corresponding organisms, and performed large-scale full-length cDNA sequencing to in-depth Learn about the function of genes. Such as: Arabidopsis (A.thaliana), mouse (M.musculus), fruit fly (D.melanoga ster), rice (O.sati2va), etc., have produced a l...

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Application Information

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IPC IPC(8): C40B40/08C40B50/06C12N15/10
Inventor 罗昊澍其他发明人请求不公开姓名
Owner BEIJING VJT BIO CO LTD
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