The Paramyxoviruses Simian Virus 5 and Mumps Virus Recruit Host Cell CD46 To Evade Complement-Mediated Neutralization

The complement system is a critical component of the innate immune response that all animal viruses must face during natural infections. Our previous results have shown that treatment of the paramyxovirus simian virus 5 (SV5) with human serum results in deposition of complement C3-derived polypeptides on virion particles. Here, we show that the virion-associated C3 component includes the inactive form iC3b, suggesting that SV5 may have mechanisms to evade the host complement system. Electron microscopy, gradient centrifugation, and Western blot analysis indicated that purified SV5 virions derived from human A549 cells contained CD46, a plasma membrane-expressed regulator of complement that acts as a cofactor for cleavage and inactivation of C3b into iC3b. In vitro cleavage assays with purified complement components showed that SV5 virions had C3b cofactor activity, resulting in specific factor I-mediated cleavage of C3b into inactive iC3b. SV5 particles generated in CHO cells, which do not express CD46, did not have cofactor activity. Conversely, virions derived from a CHO cell line that was engineered to overexpress human CD46 contained elevated levels of virion-associated CD46 and displayed enhanced C3b cofactor activity. In comparison with C3b, purified SV5 virions had very low cofactor activity against C4b, consistent with the known preference of CD46 for C3b versus C4b. Similar results were obtained for the closely related mumps virus (MuV), except that MuV particles derived from CHO-CD46 cells had higher C4b cofactor activity than SV5 virions. In neutralization assays with human serum, SV5 and MuV containing CD46 showed slower kinetics and more resistance to neutralization than SV5 and MuV that lacked CD46. Our results support a model in which the rubulaviruses SV5 and MuV incorporate cell surface complement inhibitors into progeny virions as a mechanism to limit complement-mediated neutralization.The complement system constitutes a complex group of both soluble and cell-associated proteins that together form an integral part of the innate host defense against pathogens (reviewed in references 7, 9, 11, and 31). Complement can serve to link innate and adaptive immunity through a large number of activities, including recognition of viruses, direct neutralization of infectivity, recruitment and stimulation of leukocytes, opsonization by immune cells, and activation of T- and B-cell responses (9, 11, 27). Complement activation and the ability of viruses to counteract complement can play important roles in viral pathogenesis, as well as the design of more effective vaccines and therapeutic vectors (6, 9, 17, 36, 43). The overall goal of the work described here was to determine the mechanism by which the paramyxoviruses simian virus 5 (SV5) and mumps virus (MuV) limit activation of complement pathways.The complement cascade can be initiated through three main pathways: the classical pathway, the lectin pathway, and the alternative pathway (11, 40). These three pathways converge on a central component, C3, which is activated by cleavage into C3a and C3b. C3a serves as an anaphylatoxin to promote inflammation. C3b can bind covalently to viral components to aid in opsonization and phagocytosis. In addition, C3b can associate with other factors, such as factor B, to form the C3 convertase (e.g., C3bBb), and this functions to amplify the initially deposited C3b signal by further cleavage of C3 molecules in a feedback loop. Likewise, C4 can be activated by cleavage into the anaphylatoxin C4a and the C4b fragment, which links the classical and lectin pathways with the alternative pathway. The association of C3b with components further downstream, such as C6 through C9, can lead to formation of the membrane attack complex, which is capable of lysing virus particles or infected cells (reviewed in references 7, 11, and 28).The complement system needs to be highly regulated to prevent inappropriate activation and potential damage to normal cells and healthy tissues (3). Self-regulation of complement pathways involves the highly concerted actions of a family of soluble and cell-associated proteins called regulators of complement activation (RCA). RCA proteins can limit inappropriate complement activation through two major mechanisms: (i) by accelerating the disassociation of C3 or C5 convertase or (ii) by acting as a cofactor to promote proteolytic cleavage of C3b or C4b by the complement protease factor I. Examples of RCA proteins are factor H, CD46, complement receptor 1 (CR1, or CD35), and C4 binding protein (14, 19, 24, 45).CD46, or membrane cofactor protein, is an integral membrane RCA protein that is expressed on a wide range of tissues and cell types (32). CD46 is an N- and O-linked glycosylated protein expressed at the plasma membrane as multiple isoforms that are derived from alternative splicing (32, 33, 39, 41). CD46 selectively binds to both C3b and C4b on cell surfaces, where it acts as a cofactor to promote efficient cleavage by complement protease factor I (44; reviewed in references 5 and 32). For C3b, CD46 and factor I combine to mediate inactivation to iC3b, and this is a major mechanism for limiting the amplification of low basal levels of C3b that arise from spontaneous alternative-pathway activation. CD46 also serves as a cofactor for factor I-mediated cleavage of C4b into C4c and C4d, but this cofactor activity is less efficient than that seen for C3b cleavage (35, 45).Viruses have evolved a number of mechanisms to inhibit or to delay the neutralizing effects of complement (9, 16). Large DNA viruses have coding capacities that allow them to encode a variety of mimics of host cell RCA proteins, and these viral homologs often function to inactivate complement components by supplying cofactor activity or by accelerating the decay of convertases (reviewed in references 2, 7, 29, and 31). For example, herpesvirus saimiri expresses a complement control protein that inhibits the C3 convertase (20). As an alternative mechanism to counteract complement, a number of enveloped DNA viruses and retroviruses have been shown to recruit cell-associated RCA proteins into budding particles (15, 47, 48). Examples of this are vaccinia virus and human immunodeficiency virus type 1, which incorporate CD55, CD59, and CD46 into progeny virions (16, 42, 48).In contrast to retroviruses and large DNA viruses, mechanisms that are employed to limit or evade host cell complement pathways have not been described for the paramyxovirus family of negative-strand RNA viruses (30). It has been known for many years that complement is an important factor in paramyxovirus neutralization (18, 23, 34, 49, 50). For example, the closely related paramyxoviruses SV5 and MuV preferentially activate the complement alternative pathway in vitro, and this activation can contribute to the efficiency of neutralization by human serum (23, 26). These findings raised the question of whether negative-strand RNA viruses have mechanisms to limit activation and/or amplification of the complement cascade.We have previously shown that treatment of SV5 and MuV particles with normal human serum led to deposition of C3-derived components on virions, but the virion-associated C3 molecules had properties of the inactive form, iC3b, and not the intact C3b (26). In this study, we tested the hypothesis that SV5 and MuV incorporate host cell RCA proteins into budding virions as a mechanism to limit complement activity through inactivation of C3b. CD46 was found associated with purified SV5 and MuV virions that were derived from cells expressing CD46, and these particles displayed C3b cofactor activity in vitro. Consistent with this inactivation of C3b, CD46-containing virus was more resistant to in vitro neutralization by human serum than virus derived from CD46-deficient cells. Our results support a model in which these closely related paramyxoviruses incorporate at least one cell surface RCA protein into progeny virions as a mechanism to evade complement-mediated neutralization.