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Characterization of Various Recombinant Antigens from Echinococcus multilocularis for Use in the Immunodiagnosis
Authors:Hirokazu?Kouguchi  author-information"  >  author-information__contact u-icon-before"  >  mailto:kouguchi@iph.pref.hokkaido.jp"   title="  kouguchi@iph.pref.hokkaido.jp"   itemprop="  email"   data-track="  click"   data-track-action="  Email author"   data-track-label="  "  >Email author,Tomohiro?Suzuki,Kimiaki?Yamano,Hiroshi?Honma,Yukiharu?Sawada
Affiliation:(1) Hokkaido Institute of public Health, N19, W12, Kita-Ku, Sapporo 060-0819, Japan
Abstract:Using four clones isolated from Echinococcus multilocularis cDNA library with alveolar echinococcosis (AE) patient sera, various antigens were expressed as ThioHis tag-fused protein. Recombinant EmII/3 antigen was produced as the five fragments divided into the N-terminal (#5 and #5s), the central (#6 and #6s) and the C-terminal domain (#7). Immunoblot analysis revealed that the #7 showed significant reactivity whereas those of #5 and #5s were relatively low. The #6 and #6s also showed lower reactivity than that of #7, although the two minor bands of #6 reacted with every serum. These results suggested that an immunodominant region of EmII/3 locate within the C-terminal one third. The #8s recombinant antigen, Ser23–Glu176 of actin filament fragmenting protein (AFFP), apparently reacted with the AE patient sera, while the #1 antigen synthesized as a full-length antigen B1 did not show such high reactivity. Thus, #7 and #8s antigens showed significant potential for use in immunodetection of AE. In addition, the specific antibodies against #7 and #8s reacted with specific antigens in crude extract of E. multilocularis cyst, indicating that these antigens retained antigenicity common to native EmII/3 and AFFP, respectively.
Keywords:AFFP  E. multilocularis  echinococcosis  EmII/3  recombinant antigen
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