鼠冠状病毒刺突糖蛋白的N端结构域决定了该病毒株的癌胚抗原相关细胞黏附分子1(CEACAM1)受体特异性。
The N-terminal domain of the murine coronavirus spike glycoprotein determines the CEACAM1 receptor specificity of the virus strain.
作者信息
Tsai Jean C, Zelus Bruce D, Holmes Kathryn V, Weiss Susan R
机构信息
Department of Microbiology, University of Pennsylvania School of Medicine, Philadelphia 19104, USA.
出版信息
J Virol. 2003 Jan;77(2):841-50. doi: 10.1128/jvi.77.2.841-850.2003.
Using isogenic recombinant murine coronaviruses expressing wild-type murine hepatitis virus strain 4 (MHV-4) or MHV-A59 spike glycoproteins or chimeric MHV-4/MHV-A59 spike glycoproteins, we have demonstrated the biological functionality of the N-terminus of the spike, encompassing the receptor binding domain (RBD). We have used two assays, one an in vitro liposome binding assay and the other a tissue culture replication assay. The liposome binding assay shows that interaction of the receptor with spikes on virions at 37 degrees C causes a conformational change that makes the virions hydrophobic so that they bind to liposomes (B. D. Zelus, J. H. Schickli, D. M. Blau, S. R. Weiss, and K. V. Holmes, J. Virol. 77: 830-840, 2003). Recombinant viruses with spikes containing the RBD of either MHV-A59 or MHV-4 readily associated with liposomes at 37 degrees C in the presence of soluble mCEACAM1(a), except for S(4)R, which expresses the entire wild-type MHV-4 spike and associated only inefficiently with liposomes following incubation with soluble mCEACAM1(a). In contrast, soluble mCEACAM1(b) allowed viruses with the MHV-A59 RBD to associate with liposomes more efficiently than did viruses with the MHV-4 RBD. In the second assay, which requires virus entry and replication, all recombinant viruses replicated efficiently in BHK cells expressing mCEACAM1(a). In BHK cells expressing mCEACAM1(b), only viruses expressing chimeric spikes with the MHV-A59 RBD could replicate, while replication of viruses expressing chimeric spikes with the MHV-4 RBD was undetectable. Despite having the MHV-4 RBD, S(4)R replicated in BHK cells expressing mCEACAM1(b); this is most probably due to spread via CEACAM1 receptor-independent cell-to-cell fusion, an activity displayed only by S(4)R among the recombinant viruses studied here. These data suggest that the RBD domain and the rest of the spike must coevolve to optimize function in viral entry and spread.
利用表达野生型鼠肝炎病毒4型(MHV - 4)或MHV - A59刺突糖蛋白或嵌合MHV - 4/MHV - A59刺突糖蛋白的同基因重组鼠冠状病毒,我们已经证明了刺突蛋白N端的生物学功能,该区域包含受体结合结构域(RBD)。我们使用了两种检测方法,一种是体外脂质体结合检测,另一种是组织培养复制检测。脂质体结合检测表明,在37℃下受体与病毒粒子上的刺突蛋白相互作用会引起构象变化,使病毒粒子具有疏水性,从而使其能够结合脂质体(B. D. Zelus、J. H. Schickli、D. M. Blau、S. R. Weiss和K. V. Holmes,《病毒学杂志》77: 830 - 840,2003年)。含有MHV - A59或MHV - 4的RBD的刺突蛋白的重组病毒在37℃下,在可溶性mCEACAM1(a)存在的情况下很容易与脂质体结合,但S(4)R除外,S(4)R表达整个野生型MHV - 4刺突蛋白,在与可溶性mCEACAM1(a)孵育后仅低效地与脂质体结合。相比之下,可溶性mCEACAM1(b)使具有MHV - A59 RBD的病毒比具有MHV - 4 RBD的病毒更有效地与脂质体结合。在第二种需要病毒进入和复制的检测中,所有重组病毒在表达mCEACAM1(a)的BHK细胞中都能高效复制。在表达mCEACAM1(b)的BHK细胞中,只有表达具有MHV - A59 RBD的嵌合刺突蛋白的病毒能够复制,而表达具有MHV - 4 RBD的嵌合刺突蛋白的病毒的复制则无法检测到。尽管具有MHV - 4 RBD,S(4)R仍能在表达mCEACAM1(b)的BHK细胞中复制;这很可能是由于通过不依赖CEACAM1受体的细胞间融合进行传播,在这里研究的重组病毒中只有S(4)R表现出这种活性。这些数据表明,RBD结构域和刺突蛋白的其余部分必须共同进化,以优化病毒进入和传播中的功能。
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