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BALB/c小鼠对HIV - gag的MHC I类限制性免疫反应选择了一个单一表位,该表位没有可预测的MHC结合基序,并且通过P3位的谷氨酰胺与口袋D之间的相互作用与Kd结合。

The MHC class I-restricted immune response to HIV-gag in BALB/c mice selects a single epitope that does not have a predictable MHC-binding motif and binds to Kd through interactions between a glutamine at P3 and pocket D.

作者信息

Mata M, Travers P J, Liu Q, Frankel F R, Paterson Y

机构信息

Department of Microbiology, University of Pennsylvania Medical School, Philadelphia, USA.

出版信息

J Immunol. 1998 Sep 15;161(6):2985-93.

PMID:9743362
Abstract

Using a strain of Listeria monocytogenes that stably expresses and secretes HIV gag to deliver this Ag to the MHC class I pathway of Ag processing, we have identified the immunodominant CTL epitope to gag in the BALB/c mouse and shown that it is Kd restricted. The specific motif for the peptides that bind the MHC class I molecule H-2 Kd is believed to be a nonamer with residues tyrosine or phenylalanine in the second amino acid position and leucine or isoleucine in the carboxyl-terminal or ninth amino acid position as dominant anchoring positions. Surprisingly, the identified gag peptide, AMQMLKETI, does not contain an anchoring aromatic residue in position two although competition assays with other Kd-restricted epitopes indicated that it binds to Kd with comparable affinity. Using a theoretical molecular dynamics approach to probe the stability of peptide binding to MHC class I molecules, we show that the absence of an appropriate anchor residue at P2 in AMQMLKETI is compensated by favorable interactions of the glutamine at P3 with pocket D of Kd. These findings were verified experimentally, demonstrating the predictive power of this theoretical approach in analyzing MHC class I/peptide interactions. These studies also indicate that CTL epitope prediction that relies on dominant peptide motifs may not always identify the correct epitope.

摘要

利用一种稳定表达并分泌HIV gag的单核细胞增生李斯特菌菌株,将该抗原递送至抗原加工的MHC I类途径,我们在BALB/c小鼠中鉴定出了针对gag的免疫显性CTL表位,并表明它受Kd限制。据信,与MHC I类分子H-2 Kd结合的肽的特定基序是一个九聚体,在第二个氨基酸位置有酪氨酸或苯丙氨酸残基,在羧基末端或第九个氨基酸位置有亮氨酸或异亮氨酸作为主要锚定位置。令人惊讶的是,鉴定出的gag肽AMQMLKETI在第二个位置不包含锚定芳香族残基,尽管与其他受Kd限制的表位的竞争试验表明它以相当的亲和力与Kd结合。使用理论分子动力学方法来探究肽与MHC I类分子结合的稳定性,我们表明AMQMLKETI中P2处缺乏合适的锚定残基可通过P3处的谷氨酰胺与Kd的口袋D的有利相互作用得到补偿。这些发现通过实验得到了验证,证明了这种理论方法在分析MHC I类/肽相互作用中的预测能力。这些研究还表明,依赖于主要肽基序的CTL表位预测可能并不总是能识别出正确的表位。

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