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Identification of CD8 as a peanut agglutinin (PNA) receptor molecule on immature thymocytes

机译:鉴定CD8为未成熟胸腺细胞上的花生凝集素(PNA)受体分子

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摘要

Differentiation of most T lymphocytes occurs within the thymus and is characterized by variable expression of CD4/CD8 coreceptor molecules, increased surface density of T cell antigen receptor (TCR) alpha beta proteins, and decreased expression of glycan chains recognized by the galactose-specific lectin peanut agglutinin (PNA). Although appreciated for several decades that PNA agglutination is useful for the physical separation of immature and mature thymocyte sub-populations, the identity of specific PNA-binding glycoproteins expressed on immature thymocytes remains to be determined. In the current report, we studied the expression of PNA-specific glycans on immature and mature T cells and used lectin affinity chromatography and immunoprecipitation techniques to characterize PNA-binding glycoproteins on thymocytes. Our data demonstrate that PNA-specific glycans are localized on a relatively small subset of thymocyte surface proteins, several of which were specifically identified, including CD43, CD45, and suprisingly, CD8 molecules. CD8 alpha and CD8 alpha' proteins bound to PNA in the absence of CD8 beta expression showing that O-glycans on CD8 beta glycoproteins are not necessary for PNA binding and that glycosylation of CD8 alpha and CD8 alpha' proteins proceeds effectively in the absence of CD8 beta. Finally, we demonstrate that PNA binding of CD8 is developmentally regulated by sialic acid addition as CD8 proteins from mature T cells bound to PNA only after sialidase treatment. These studies identify CD8 as a PNA receptor molecule on immature thymocytes and show that PNA binding of CD8 on immature and mature T cells is developmentally regulated by sialic acid modification.
机译:大多数T淋巴细胞的分化发生在胸腺内,其特征在于CD4 / CD8共受体分子的可变表达,T细胞抗原受体(TCR)αβ蛋白的表面密度增加以及半乳糖特异性凝集素识别的聚糖链的表达降低花生凝集素(PNA)。尽管几十年来人们认识到PNA凝集可用于物理分离未成熟和成熟的胸腺细胞亚群,但在未成熟胸腺细胞上表达的特异性PNA结合糖蛋白的身份仍有待确定。在本报告中,我们研究了未成熟和成熟T细胞上PNA特异性聚糖的表达,并使用了凝集素亲和层析和免疫沉淀技术来表征胸腺细胞上PNA结合糖蛋白。我们的数据表明,PNA特异性聚糖位于胸腺细胞表面蛋白的一个相对较小的子集上,其中有几个是经过专门鉴定的,包括CD43,CD45和令人惊讶的CD8分子。在没有CD8 beta表达的情况下,CD8 alpha和CD8 alpha'蛋白与PNA结合,表明CD8 beta糖蛋白上的O-聚糖对于PNA结合不是必需的,并且在没有CD8的情况下,CD8 alpha和CD8 alpha'蛋白的糖基化有效进行Beta。最后,我们证明CD8的PNA结合受到唾液酸添加的调控,因为成熟T细胞中的CD8蛋白仅在唾液酸酶处理后才与PNA结合。这些研究将CD8鉴定为未成熟胸腺细胞上的PNA受体分子,并表明未成熟和成熟T细胞上CD8的PNA结合受到唾液酸修饰的发育调控。

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