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牛 CD46 的遗传和剪接变异使细胞对牛病毒性腹泻病毒(牛瘟病毒)的易感性发生转移。

Genetic and splice variations of Bos taurus CD46 shift cell permissivity to BVDV, the bovine pestivirus.

机构信息

Department of Morphology and Pathology, Faculty of Veterinary Medicine, University of Liège, Sart Tilman B43, Belgium.

出版信息

Vet Microbiol. 2011 Sep 28;152(3-4):315-27. doi: 10.1016/j.vetmic.2011.05.028. Epub 2011 May 25.

DOI:10.1016/j.vetmic.2011.05.028
PMID:21680116
Abstract

The pestivirus bovine viral diarrhea virus (BVDV) is known to bind to the CD46 molecule, which subsequently promotes entry of the virus. Mapping of the BVD-virion-binding site has shown that two peptides, 66EQIV69 and 82GQVLAL87, located on antiparallel beta sheets in the most distal complement control protein module (CCP1), provide the attachment platform. In the present study, we reveal the existence of ten distinct allelic versions of the CCP1 module, varying significantly in frequency among taurine and indicine races. A complex mRNA splicing pattern was also evidenced for bovine CD46, generating three different serine-threonine-proline segments and five different cytoplasmic domains. The four most frequent allelic variants and the six splice variants were then expressed in BVDV-nonpermissive porcine cells and the quantity of progeny virions generated by each cell preparation was measured 48 h post-infection. As expected, ectopic expression of the 10 bovine CD46 isoforms rendered the PK15 cells permissive to BVDV, as attested by the 100,000-fold greater recovery of virions from these cells than from non-transfected cells. This permissivity increase was significantly lower (-33%, P<0.001) when the canonical CCP1 was replaced with the variant most frequent in zebus, suggesting positive or negative selection of this allele in the latter and in the former, respectively. The predicted secondary structure of this variant suggests that the measured loss of function is due to the disappearance of one of the two beta sheets constituting the BVDV attachment platform. On the other hand we showed that for a given CCP1, the titer recovered at 48 hpi also depended on the nature of the CD46 cytoplasmic domain (P<0.001). This result implies that virus binding generates a cytoplasmic-tail-dependent outside-in signal that determines permissivity to BVDV.

摘要

牛病毒性腹泻病毒(BVDV)已知能与 CD46 分子结合,随后促进病毒进入。BVDV 病毒结合位点的定位表明,位于最远端补体控制蛋白模块(CCP1)的两个反平行β片层上的两个肽段 66EQIV69 和 82GQVLAL87 提供了附着平台。在本研究中,我们揭示了 CCP1 模块存在十种不同的等位基因变体,在牛科和牛科之间的频率有很大差异。还证明了牛 CD46 的复杂 mRNA 剪接模式,生成了三个不同的丝氨酸-苏氨酸-脯氨酸片段和五个不同的细胞质结构域。然后,将这四种最常见的等位基因变体和六种剪接变体在 BVDV 非允许的猪细胞中表达,并在感染后 48 小时测量每个细胞制备物产生的后代病毒粒子的数量。如预期的那样,10 种牛 CD46 同工型的异位表达使 PK15 细胞对 BVDV 具有允许性,这证明从这些细胞中回收的病毒粒子比从未转染的细胞中回收的病毒粒子多 100000 倍。当用在印度野牛中最常见的变体替换经典的 CCP1 时,这种允许性的增加显著降低(-33%,P<0.001),这表明在后者和前者中,该等位基因分别受到正选择或负选择。该变体的预测二级结构表明,所测量的功能丧失是由于构成 BVDV 附着平台的两个β片层之一的消失。另一方面,我们表明,对于给定的 CCP1,在 48 hpi 回收的滴度也取决于 CD46 细胞质结构域的性质(P<0.001)。这一结果意味着病毒结合产生了一种依赖细胞质尾巴的外向信号,决定了对 BVDV 的允许性。

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