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微小泰勒虫150 kDa微球体抗原的克隆与特性分析,该抗原与多态性免疫显性分子(PIM)存在免疫交叉反应。

Cloning and characterization of a 150 kDa microsphere antigen of Theileria parva that is immunologically cross-reactive with the polymorphic immunodominant molecule (PIM).

作者信息

Skilton R A, Bishop R P, Wells C W, Spooner P R, Gobright E, Nkonge C, Musoke A J, Macklin M, Iams K P

机构信息

International Livestock Research Institute (ILRI), Nairobi, Kenya.

出版信息

Parasitology. 1998 Oct;117 ( Pt 4):321-30. doi: 10.1017/s0031182098003163.

Abstract

To identify the genes encoding novel immunodominant antigens of Theileria parva a lambda gt11 library of piroplasm genomic DNA was immunoscreened with bovine recovery serum and a gene encoding a 150 kDa antigen (p150) was identified. The predicted polypeptide contains an N-terminal secretory signal sequence and a proline-rich region of repeated amino acid motifs. The repeat region is polymorphic between stocks of T. parva in both copy number and sequence, and analysis of the repeat region from 10 stocks of T. parva revealed 5 p150 variants. A monoclonal antibody (mAb) against the T. parva polymorphic immunodominant molecule (PIM) cross-reacted with the recombinant p150. The p150 has sequence homology with a PIM peptide sequence containing the anti-PIM mAb epitope. Immunoelectron microscopy demonstrated that the p150 antigen, like PIM, is located in the microspheres of the sporozoites and is exocytosed following sporozoite invasion of the host lymphocyte. By immunoelectron microscopy p150 was subsequently transiently detectable on the sporozoite surface and in the lymphocyte cytosol. Immunoblotting showed that p150 is also expressed by the schizont stage, but at much lower levels compared to the sporozoite. These results suggest a major role for p150 in the early events of host-sporozoite interaction.

摘要

为了鉴定编码微小泰勒虫新型免疫显性抗原的基因,用牛恢复血清对梨形虫基因组DNA的λgt11文库进行免疫筛选,鉴定出一个编码150 kDa抗原(p150)的基因。预测的多肽包含一个N端分泌信号序列和一个富含脯氨酸的重复氨基酸基序区域。重复区域在微小泰勒虫不同虫株之间的拷贝数和序列上具有多态性,对10个微小泰勒虫虫株的重复区域分析揭示了5种p150变体。一种针对微小泰勒虫多态性免疫显性分子(PIM)的单克隆抗体(mAb)与重组p150发生交叉反应。p150与包含抗PIM mAb表位的PIM肽序列具有序列同源性。免疫电子显微镜显示,p150抗原与PIM一样,位于子孢子的微球中,并在子孢子侵入宿主淋巴细胞后被胞吐。通过免疫电子显微镜观察,随后在子孢子表面和淋巴细胞胞质溶胶中短暂检测到p150。免疫印迹显示,p150在裂殖体阶段也有表达,但与子孢子相比表达水平要低得多。这些结果表明p150在宿主-子孢子相互作用的早期事件中起主要作用。

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