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EPITOPE MAPPING OF THE V3 DOMAIN OF FELINE IMMUNODEFICIENCY VIRUS ENVELOPE GLYCOPROTEIN BY MONOCLONAL-ANTIBODIES

机译:单克隆抗体对猫免疫缺陷病毒包膜糖蛋白V3域的表位作图

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摘要

A panel of six IgG monoclonal antibodies (MAbs) was produced by immunizing mice with a 22 amino acid synthetic peptide, designated V3.3, of the third variable region of feline immunodeficiency virus (FIV) envelope glycoprotein. This peptide is known to induce neutralizing antibodies in cats. In ELISA all MAbs reacted with purified SDS-disrupted FIV and in flow cytometry all MAbs stained permeated, persistently infected FL4 cells but not unfixed FL4 cells; this indicated that the MAbs recognize essentially cryptic epitopes of the gp100 V3 loop. By direct ELISA using partially overlapping synthetic peptides and by competition binding studies, the anti-V3.3 MAbs were shown to detect at least four distinct epitopes, two located in the amino-terminal half and two in the carboxy-terminal half of the sequence. When tested for neutralizing activity by the syncytium inhibition assay in Crandell feline kidney cells, all anti-V3.3 MAbs neutralized FIV at high dilution. However, at low dilution two MAbs exhibited much less neutralizing activity. These results indicate that the V3 region of FIV contains multiple epitopes involved in neutralization.
机译:通过用22个氨基酸的猫免疫缺陷病毒(FIV)包膜糖蛋白第三可变区的合成肽(称为V3.3)免疫小鼠,产生了一组六种IgG单克隆抗体(MAb)。已知该肽可诱导猫中和抗体。在ELISA中,所有MAb与纯化的SDS破坏的FIV反应,在流式细胞仪中,所有MAbs染色渗透,持续感染的FL4细胞,但未固定的FL4细胞不染色;这表明,MAb基本上识别gp100 V3环的隐秘表位。通过使用部分重叠的合成肽的直接ELISA以及竞争结合研究,抗V3.3 MAb被证明可检测至少四个不同的表位,其中两个位于序列的氨基末端一半,而两个位于羧基末端一半。当通过Crandell猫肾细胞中的合胞体抑制测定法测试中和活性时,所有抗V3.3 MAb均以高稀释度中和了FIV。但是,在低稀释度下,两种单克隆抗体的中和活性要低得多。这些结果表明FIV的V3区域含有参与中和的多个表位。

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