Fractionation of respiratory syncytial (RS) virus components by centrifugation techniques

During the course of 26 respiratory syncytial (RS) virus infections, infected cells in the respiratory tract become coated with immunoglobulins (IgA, IgG, and IgM), IgA being predominant. Methods are described for detecting both intracellular virus and coating immunoglobulin using a double staining

## Abstract Lymphocyte proliferation assays were used to determine the ability of human and BALB/c T‐ lymphocytes to recognise and respond to in vitro challenge with purified preparations of four res piratory syncytial (RS) virus proteins. Human peripheral blood lymphocytes (PBLs) collected from ad

The IgG-subclass specific antibody response was investigated in primary RS-virus infections in infants and small children by using an ELISA with monoclonal antibodies against the four human IgG subclasses. When 78 serum samples obtained from 21 patients during the first 3-4 mo following the onset of

## Abstract Samples of nasopharyngeal secretions (NPS) obtained from 140 infants and children with acute respiratory disease were examined for the presence of respiratory syncytial (RS) virus by ELISA. An antiserum produced in rabbits against RS‐virus polypeptides was used both as the “capture” ant

The presence of respiratory syncytial virus (RSV) was investigated by immunofluorescent antibody (IF) technique and by a biotidavidin (BA) ELISA in 156 samples of nasopharyngeal secretions (NPS) obtained from infants and small children with acute respiratory disease. Of 70 RSV-IF-positive NPS, 68 we