| Literature DB >> 16098216 |
Blanquita B De Guzman1, Junzo Hisatsune, Masaaki Nakayama, Kinnosuke Yahiro, Akihiro Wada, Eiki Yamasaki, Yoshito Nishi, Shiho Yamazaki, Takeshi Azuma, Yoshiyuki Ito, Masahiro Ohtani, Thea van der Wijk, Jeroen den Hertog, Joel Moss, Toshiya Hirayama.
Abstract
Helicobacter pylori vacuolating cytotoxin, VacA, induces vacuolation in mammalian cell lines. Sequence differences in the middle of VacA molecules define two families, termed m1VacA and m2VacA, which differ in cell specificity. Similar to m1VacA, m2VacA is activated by acid or alkali, which enhances its binding to cells. Immunoprecipitation experiments showed that, in AZ-521 cells, activated m2VacA, similar to m1VacA, binds to two receptor-like protein tyrosine phosphatases, RPTPalpha and RPTPbeta suggesting that activated m2VacA as well as m1VacA may contribute to gastrointestinal disease following H. pylori infection. G401 cells express RPTPalpha, not RPTPbeta, and responded to both m1VacA and m2VacA. HeLa cells likewise expressed RPTPalpha, not RPTPbeta, but, in contrast to other cell lines, responded poorly to m2VacA. m1VacA associated with RPTPalpha of HeLa cells to an extent similar to that in other toxin-sensitive cells, whereas activated m2VacA bound HeLa cell RPTPalpha less well, consistent with its low vacuolating activity against these cells. The molecular mass of RPTPalpha from HeLa cells is less than that of the protein from G401 cells, although their extracellular amino acid sequences are virtually identical, with only two amino acid differences noted. Different post-translational modifications of RPTPalpha in HeLa cells may be responsible for the reduced susceptibility to m2VacA.Entities:
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Year: 2005 PMID: 16098216 DOI: 10.1111/j.1462-5822.2005.00556.x
Source DB: PubMed Journal: Cell Microbiol ISSN: 1462-5814 Impact factor: 3.715