Ban J, Portetelle D, Altaner C, Horion B, Milan D, Krchnak V, Burny A, Kettmann R
Department of Molecular Virology, Slovak Academy of Sciences, Bratislava.
J Virol. 1993 Feb;67(2):1050-7. doi: 10.1128/JVI.67.2.1050-1057.1993.
An immunoscreening strategy was used to isolate a cDNA clone encoding the binding domain for the external glycoprotein gp51 of the bovine leukemia virus (BLV). Three recombinant phages demonstrating BLV binding activity and containing 2.3-kbp cDNA inserts with identical nucleotide sequences were isolated from a lambda gt11 cDNA library of bovine kidney cells (MDBK). One clone, BLVRcp1, hybridized with a 4.8-kb mRNA from cells of bovine origin and was also found to be conserved as a single-copy gene in murine, bovine, ovine, primate, canine, feline, and porcine DNAs. The same gene is amplified in caprine DNA isolated from a BLV-induced tumor. The longest open reading frame of BLVRcp1 encodes a protein fragment of 729 amino acids with a putative receptor structure. BLVRcp1 cDNA was cloned in the eucaryotic expression vector pXT-1 and transfected into murine NIH 3T3 and human HEp-2 cells. Cells expressing BLVRcp1 mRNA became susceptible to BLV infection. BLVRcp1 has no known physiological function and has no significant homology with sequences registered in the GenBank and EMBL data libraries (31 July 1992). Expression of deleted constructs of BLVRcp1 indicates that the BLV binding region is encoded at the 5' side of the receptor clone.
采用免疫筛选策略分离出一个编码牛白血病病毒(BLV)外膜糖蛋白gp51结合结构域的cDNA克隆。从牛肾细胞(MDBK)的λgt11 cDNA文库中分离出三个具有BLV结合活性、含有2.3-kbp cDNA插入片段且核苷酸序列相同的重组噬菌体。其中一个克隆BLVRcp1与源自牛细胞的4.8-kb mRNA杂交,并且发现在小鼠、牛、绵羊、灵长类、犬科、猫科和猪的DNA中作为单拷贝基因保守存在。从BLV诱导的肿瘤中分离的山羊DNA中也扩增出相同的基因。BLVRcp1最长的开放阅读框编码一个具有推定受体结构的729个氨基酸的蛋白质片段。将BLVRcp1 cDNA克隆到真核表达载体pXT-1中,并转染到小鼠NIH 3T3细胞和人HEp-2细胞中。表达BLVRcp1 mRNA的细胞变得易受BLV感染。BLVRcp1没有已知的生理功能,与1992年7月31日GenBank和EMBL数据库中登记的序列没有显著同源性。BLVRcp1缺失构建体的表达表明BLV结合区域在受体克隆的5'端编码。
