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食蟹猴和狒狒透明带蛋白的克隆与表达。

Cloning and expression of cynomolgus monkey and baboon zona pellucida proteins.

作者信息

Harris Jeffrey D, Piersen Colleen E

机构信息

Zonagen, Inc., The Woodlands, Texas 77380, USA.

出版信息

Mol Reprod Dev. 2003 Jul;65(3):237-44. doi: 10.1002/mrd.10288.

DOI:10.1002/mrd.10288
PMID:12784244
Abstract

Partial clones for the three cynomolgus monkey (Macaca fasicularis) zona pellucida genes (cmZPA, cmZPB, and cmZPC) have previously been isolated. These partial clones contained the sequences for the C-terminal portion of each rcmZP protein. To obtain full-length clones for each cmZP, a fresh cynomolgus monkey ovarian cDNA library was constructed. PCR methodology was employed to speed the isolation of full-length clones for each cmZP cDNA. The 3' primers were designed based on sequence information from the previously identified clones; the 5' primers were designed using the human ZP sequences. The PCR technique yielded full-length clones of cmZPA and cmZPC, but not of cmZPB. Therefore, a genomic clone of cmZPB was isolated and the sequence determined. The exon/intron structure is nearly identical to the human ZPB exon/intron structure. New PCR primers were designed based on the cynomolgus monkey ZPB genomic sequence, and a full-length cmZPB cDNA was obtained. The same primers that were used to generate the cmZPB were also used to generate a baboon (Papio cynocephalus) ZPB (bZPB) cDNA. As was done previously for the human zona pellucida (hZP) cDNAs, the cmZP, and bZPB cDNAs were transferred to shuttle vectors for transfection into Chinese Hamster Ovary (CHO) cells. Stable cell lines for producing each ZP protein were isolated. Each cell line secreted the desired recombinant zona pellucida (rZP) protein into the culture medium, and each protein was purified using an established protocol. In terms of size and purity, the purified recombinant cmZP (rcmZP) and rbZPB proteins resemble the rhZP proteins.

摘要

先前已分离出三种食蟹猴(猕猴)透明带基因(cmZPA、cmZPB和cmZPC)的部分克隆。这些部分克隆包含每个rcmZP蛋白C末端部分的序列。为了获得每个cmZP的全长克隆,构建了一个新的食蟹猴卵巢cDNA文库。采用PCR方法加速每个cmZP cDNA全长克隆的分离。3'引物是根据先前鉴定的克隆的序列信息设计的;5'引物是使用人ZP序列设计的。PCR技术产生了cmZPA和cmZPC的全长克隆,但没有产生cmZPB的全长克隆。因此,分离出cmZPB的基因组克隆并确定了其序列。外显子/内含子结构与人类ZPB外显子/内含子结构几乎相同。根据食蟹猴ZPB基因组序列设计了新的PCR引物,并获得了全长cmZPB cDNA。用于生成cmZPB的相同引物也用于生成狒狒(东非狒狒)ZPB(bZPB)cDNA。如同先前对人透明带(hZP)cDNA所做的那样,将cmZP和bZPB cDNA转移到穿梭载体中,用于转染中国仓鼠卵巢(CHO)细胞。分离出了用于产生每种ZP蛋白的稳定细胞系。每个细胞系将所需的重组透明带(rZP)蛋白分泌到培养基中,并且每种蛋白都使用既定方案进行了纯化。就大小和纯度而言,纯化的重组cmZP(rcmZP)和rbZPB蛋白类似于rhZP蛋白。

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