Callaway Heather M, Feng Kurtis H, Lee Donald W, Allison Andrew B, Pinard Melissa, McKenna Robert, Agbandje-McKenna Mavis, Hafenstein Susan, Parrish Colin R
Baker Institute for Animal Health, Department of Microbiology and Immunology, College of Veterinary Medicine, Cornell University, Ithaca, New York, USA.
School of Chemical and Biomolecular Engineering, Cornell University, Ithaca, New York, USA.
J Virol. 2017 Jan 3;91(2). doi: 10.1128/JVI.01871-16. Print 2017 Jan 15.
Parvovirus capsids are small but complex molecular machines responsible for undertaking many of the steps of cell infection, genome packing, and cell-to-cell as well as host-to-host transfer. The details of parvovirus infection of cells are still not fully understood, but the processes must involve small changes in the capsid structure that allow the endocytosed virus to escape from the endosome, pass through the cell cytoplasm, and deliver the single-stranded DNA (ssDNA) genome to the nucleus, where viral replication occurs. Here, we examine capsid substitutions that eliminate canine parvovirus (CPV) infectivity and identify how those mutations changed the capsid structure or altered interactions with the infectious pathway. Amino acid substitutions on the exterior surface of the capsid (Gly299Lys/Ala300Lys) altered the binding of the capsid to transferrin receptor type 1 (TfR), particularly during virus dissociation from the receptor, but still allowed efficient entry into both feline and canine cells without successful infection. These substitutions likely control specific capsid structural changes resulting from TfR binding required for infection. A second set of changes on the interior surface of the capsid reduced viral infectivity by >100-fold and included two cysteine residues and neighboring residues. One of these substitutions, Cys270Ser, modulates a VP2 cleavage event found in ∼10% of the capsid proteins that also was shown to alter capsid stability. A neighboring substitution, Pro272Lys, significantly reduced capsid assembly, while a Cys273Ser change appeared to alter capsid transport from the nucleus. These mutants reveal additional structural details that explain cell infection processes of parvovirus capsids.
Parvoviruses are commonly found in both vertebrate and invertebrate animals and cause widespread disease. They are also being developed as oncolytic therapeutics and as gene therapy vectors. Most functions involved in infection or transduction are mediated by the viral capsid, but the structure-function correlates of the capsids and their constituent proteins are still incompletely understood, especially in relation to identifying capsid processes responsible for infection and release from the cell. Here, we characterize the functional effects of capsid protein mutations that result in the loss of virus infectivity, giving a better understanding of the portions of the capsid that mediate essential steps in successful infection pathways and how they contribute to viral infectivity.
细小病毒衣壳虽小却是复杂的分子机器,负责执行细胞感染、基因组包装以及细胞间和宿主间转移等许多步骤。细胞感染细小病毒的具体细节仍未完全了解,但这些过程必然涉及衣壳结构的微小变化,使被内吞的病毒能够从内体逃逸,穿过细胞质,并将单链DNA(ssDNA)基因组递送至细胞核,在细胞核中发生病毒复制。在此,我们研究了消除犬细小病毒(CPV)感染性的衣壳替换情况,并确定这些突变如何改变衣壳结构或改变与感染途径的相互作用。衣壳外表面的氨基酸替换(Gly299Lys/Ala300Lys)改变了衣壳与1型转铁蛋白受体(TfR)的结合,尤其是在病毒从受体解离过程中,但仍能使病毒高效进入猫和犬细胞却无法成功感染。这些替换可能控制了感染所需的由TfR结合导致的特定衣壳结构变化。衣壳内表面的第二组变化使病毒感染性降低了100倍以上,其中包括两个半胱氨酸残基及其相邻残基。这些替换之一,Cys270Ser,调节了约10%的衣壳蛋白中出现的VP2切割事件,该事件也被证明会改变衣壳稳定性。相邻的替换Pro272Lys显著降低了衣壳组装,而Cys273Ser的变化似乎改变了衣壳从细胞核的转运。这些突变体揭示了更多解释细小病毒衣壳细胞感染过程的结构细节。
细小病毒常见于脊椎动物和无脊椎动物中,并引发广泛疾病。它们也正被开发用于溶瘤治疗和作为基因治疗载体。感染或转导中涉及的大多数功能由病毒衣壳介导,但衣壳及其组成蛋白的结构 - 功能关系仍未完全了解,特别是在确定负责感染和从细胞释放的衣壳过程方面。在此,我们表征了导致病毒感染性丧失的衣壳蛋白突变的功能影响,从而更好地理解衣壳中介导成功感染途径中关键步骤的部分以及它们如何影响病毒感染性。
