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斑点叉尾鮰可溶性 FcmuR 结合 Cmu3 和 Cmu4 上存在的保守线性表位。

Channel catfish soluble FcmuR binds conserved linear epitopes present on Cmu3 and Cmu4.

机构信息

Department of Microbiology, University of Mississippi Medical Center, Jackson, MS 39216, USA.

出版信息

Mol Immunol. 2010 Mar;47(6):1306-16. doi: 10.1016/j.molimm.2009.11.026. Epub 2009 Dec 23.

Abstract

A linear epitope on catfish IgM has been identified as the docking site for the catfish soluble FcmuR (IpFcRI). Western blot analyses and latex bead binding assays identified the consensus octapeptide motif FxCxVxHE located at the second cysteine that forms the intrachain disulfide bond of the catfish Cmu3 and Cmu4 immunolglobulin (Ig) domains as the IpFcRI binding sites. Furthermore, molecular modeling of catfish Cmu3 and Cmu4 confirmed that the octapeptide in both of these domains is accessible for IpFcRI interactions. In addition, since this octapeptide motif is also found in other vertebrate Ig domains, IpFcRI binding to Ig heavy (H) and light (L) chains from rainbow trout, chicken, mouse, rabbit, and goat were examined by Western blot analyses and latex bead binding assays. IpFcRI readily bound reduced rainbow trout (Igmu), chicken (Ignu), mouse (Igmu, Iggamma1, Iggamma2a, Iggamma2b, and Igalpha), rabbit (Igmu and Iggamma) and goat (Iggamma) IgH chains, and mouse Igkappa and Iglambda, and chicken Iglambda IgL chains. IpFcRI also bound mouse IgM, IgA and IgG subclasses when examined under native conditions.

摘要

已鉴定出鲶鱼 IgM 上的线性表位是鲶鱼可溶性 FcmuR(IpFcRI)的对接位点。Western blot 分析和乳胶珠结合试验鉴定出位于第二个半胱氨酸的共识八肽基序 FxCxVxHE,该半胱氨酸形成鲶鱼 Cmu3 和 Cmu4 免疫球蛋白(Ig)结构域内的二硫键,是 IpFcRI 的结合位点。此外,鲶鱼 Cmu3 和 Cmu4 的分子建模证实,这两个结构域中的八肽都可与 IpFcRI 相互作用。此外,由于该八肽基序也存在于其他脊椎动物 Ig 结构域中,因此通过 Western blot 分析和乳胶珠结合试验检查了 IpFcRI 与虹鳟鱼、鸡、鼠、兔和山羊的 Ig 重(H)链和轻(L)链的结合。IpFcRI 可轻易结合还原的虹鳟鱼(Igmu)、鸡(Ignu)、鼠(Igmu、Iggamma1、Iggamma2a、Iggamma2b 和 Igalpha)、兔(Igmu 和 Iggamma)和山羊(Iggamma)的 IgH 链,以及鼠的 Igkappa 和 Iglambda,和鸡的 Iglambda IgL 链。IpFcRI 在天然条件下也可结合鼠 IgM、IgA 和 IgG 亚类。

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