Abstract
BackgroundAdhesion of Mycoplasma pneumoniae (M. pneumoniae) to host epithelial cells requires several adhesin proteins like P1, P30 and P116. Among these proteins, P1 protein has been inedited as one of the major adhesin and immunogenic protein present on the attachment organelle of M. pneumoniae. In the present study, we scanned the entire sequence of M. pneumoniae P1 protein to identify the immunodominant and cytadherence region(s). M. pneumoniae P1 gene was synthesized in four segments replacing all the UGA codons to UGG codons. Each of the four purified P1 protein fragment was analyzed for its immunogenicity with anti-M. pneumoniae M129 antibodies (Pab M129) and sera of M. pneumoniae infected patients by western blotting and ELISA. Antibodies were produced against all the P1 protein fragments and these antibodies were used for M. pneumoniae adhesion, M. pneumoniae adhesion inhibition and M. pneumoniae surface exposure assays using HEp-2 cells lines.ResultsOur results show that the immunodominant regions are distributed throughout the entire length of P1 protein, while only the N- and C- terminal region(s) of P1 protein are surface exposed and block cytadhesion to HEp-2 cells, while antibodies to two middle fragments failed to block cytadhesion.ConclusionsThese results have important implications in designing strategies to block the attachment of M. pneumoniae to epithelial cells, thus preventing the development of atypical pneumonia.
Highlights
Adhesion of Mycoplasma pneumoniae (M. pneumoniae) to host epithelial cells requires several adhesin proteins like P1, P30 and P116
M. pneumoniae is found to be associated with other respiratory tract infections such as tracheobronchitis, bronchiolitis, croup, Acute Respiratory Distress Syndrome (ARDS), Guillain-Barre Syndrome (GBS), stroke and less severe upper respiratory tract infections in older children as well
Previous reports and we have shown that a C-terminal region of P1 antigen can comparably diagnose M. pneumoniae infection taking the SerionVirion ELISA as the standard [14,21]
Summary
Adhesion of Mycoplasma pneumoniae (M. pneumoniae) to host epithelial cells requires several adhesin proteins like P1, P30 and P116. Among these proteins, P1 protein has been inedited as one of the major adhesin and immunogenic protein present on the attachment organelle of M. pneumoniae. Each of the four purified P1 protein fragment was analyzed for its immunogenicity with anti-M. pneumoniae M129 antibodies (Pab M129) and sera of M. pneumoniae infected patients by western blotting and ELISA. Cytadherence requires a complex interaction of several M. pneumoniae proteins present on the attachment organelle, including the adhesins P1 (170 kDa), P30 (30 kDa), and P116 (116 kDa) and proteins HMW1 to HMW3, as well as proteins A, B and C [4,10,11,12,13,14,15]. Serum samples from patients suffering from M. pneumoniae infection have been shown to bind the peptide fragments located in the middle of the ~170 kDa P1 antigens [22]
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