Cytoplasmic inclusions in respiratory syncytial virus-infected cells comprising viral nucleocapsid proteins (L,N
Respiratory syncytial virus (RSV), a member of the familyParamyxoviridae, is one of the most important viral agents causing lower respiratory tract disease in infants, the elderly, and immunocompromised patients of all ages (3, 6, 21). The genome of RSV is a nonsegmented negative-strand RNA encoding 11 proteins (3). In RSV-infected cells, the viral RNA with the L (polymerase), N (nucleocapsid), P (phosphoprotein), and M2-1 proteins form the polymerase complex in which the transcription of messenger and genomic RNA takes place. As the cytoplasmic inclusions in RSV-infected cells have been shown to contain all elements of the polymerase complex and are capable of transcription in isolation (1, 7), it is presumed that they are major sites of viral transcription.Several studies have shown that the N protein is the major driver for the formation of these cytoplasmic inclusions. N associates with viral RNA, and N-RNA complexes are resistant to RNase treatment (18). Inclusion-like structures are formed when the N and P proteins are coexpressed in cells (7), and this association results from a specific protein-protein interaction between N and P, which can be disrupted by mutagenesis (8, 24). Garcia et al. (7) also showed that the M2-1 protein is present in cytoplasmic inclusions; subsequent investigations confirmed that the association of the M2-1 protein with inclusions resulted from its association with P (16).We previously reported that the RSV M protein is also found in cytoplasmic inclusions late during infection, in association with the N, P, and M2-1 proteins (11). Since we have also shown that the M protein inhibits virus transcription (11), the role of the M protein in cytoplasmic inclusions may be to inhibit viral transcription as a prelude to viral assembly and budding, driven by the M protein bringing cytoplasmic nucleocapsids into association with RSV envelope proteins (10). The concept is supported by data indicating specific interactions between M and the cytoplasmic domains of envelope glycoproteins (10).To date, it is not known how M becomes associated with the nucleocapsid complex. In the current study, we demonstrate that the N terminus of M can bind directly to M2-1 in a cell-free assay and that M colocalizes with M2-1 in the cytoplasm of cells either infected with RSV or expressing only M and M2-1 proteins. Using a cotransfection system, it was demonstrated that M associates with inclusion-like structures formed by N and P only in the presence of M2-1.
MATERIALS AND METHODS
Cells and virus.Human epithelial (HEp2) cells were grown in Dulbecco's modified Eagle's medium supplemented with 10% fetal calf serum (FCS) at 37°C and 5% CO 2 . RSV subgroup A strain A2 (a gift from Paul Young, University of Queensland, Brisbane, Australia) was grown in HEp2 cells as previously described (9). To prepare the virus stock, an 80% confluent cell monolayer was infected with RSV at a multiplicity of infect...
