Romero P, Eberl G, Casanova J L, Cordey A S, Widmann C, Luescher I F, Corradin G, Maryanski J L
Ludwig Institute for Cancer Research, Lausanne Branch, Epalinges, Switzerland.
J Immunol. 1992 Mar 15;148(6):1871-8.
In the present study, we have explored ways of inducing a CTL response to a previously defined H-2Kd MHC class I restricted epitope in the circumsporozoite (CS) protein of Plasmodium berghei, and studied in detail the fine specificity of the response. We found that the s.c. injection of a variety of synthetic peptides emulsified in Freund's adjuvant efficiently induced a specific CTL response in (BALB/c x C57BL/6)F1 (H-2d x H-2b) mice. In contrast, BALB/c mice responded only marginally, consistent with the possible requirement for a concomitant Th response that would be provided by the C57BL/6 strain. Similar to our previous observations in analyzing CTL clones from sporozoite-immunized mice, the CTL response induced by peptide immunization was in part cross-reactive with an epitope from the Plasmodium yoelii species. The minimal P. berghei CS epitope, the octapeptide PbCS 253-260, was studied in detail by the analysis of a series of variant CS peptides containing single Ala substitutions. The relative antigenic activity for each variant peptide was calculated for 28 different CTL clones. Overall, the response to this P. berghei CTL epitope appeared to be extremely diverse in terms of fine specificity. This was evident among the CTL derived from sporozoite-immunized mice, as well as among those from peptide-immunized animals. The heterogeneity found at the functional level correlates with the highly diverse TCR repertoire that we have found for the same series of CTL clones in a study that is reported separately. The relative competitor activity for each Ala-substituted peptide was also determined in a quantitative functional competition assay. For the residues (Tyr253 and Ile260) within the 8-mer CS peptide, substitution with Ala reduced competitor activity by at least 40-fold, and for two others the reduction was 5- to 10-fold. When the relative antigenic activity for each CTL/peptide combination was normalized to the relative competitor activity of the peptide, a striking pattern emerged. The two residues that most affected competitor activity showed no additional effect on recognition beyond that observed for competition. In marked contrast, Ala substitutions at the other five positions tested varied widely, depending on the CTL/peptide combination. This pattern not only supports a model whereby the Tyr253 and Ile260 residues anchor the peptide to the Kd molecule, but also implies that they are virtually inaccessible to the TCR.
在本研究中,我们探索了诱导对伯氏疟原虫环子孢子(CS)蛋白中先前定义的H-2Kd MHC I类限制性表位产生CTL反应的方法,并详细研究了该反应的精细特异性。我们发现,皮下注射多种在弗氏佐剂中乳化的合成肽能有效地在(BALB/c×C57BL/6)F1(H-2d×H-2b)小鼠中诱导特异性CTL反应。相比之下,BALB/c小鼠的反应很微弱,这与可能需要C57BL/6品系提供的伴随Th反应一致。与我们之前分析来自子孢子免疫小鼠的CTL克隆的观察结果相似,肽免疫诱导的CTL反应部分与约氏疟原虫物种的一个表位交叉反应。通过分析一系列含有单个丙氨酸替代的变体CS肽,对最小的伯氏疟原虫CS表位八肽PbCS 253-260进行了详细研究。计算了28个不同CTL克隆对每个变体肽的相对抗原活性。总体而言,对该伯氏疟原虫CTL表位的反应在精细特异性方面似乎极其多样。这在源自子孢子免疫小鼠的CTL中以及肽免疫动物的CTL中都很明显。在功能水平上发现的异质性与我们在另一项单独报道的研究中为同一系列CTL克隆发现的高度多样的TCR库相关。还通过定量功能竞争试验确定了每个丙氨酸替代肽的相对竞争活性。对于8聚体CS肽中的残基(Tyr253和Ile260),用丙氨酸替代使竞争活性降低至少40倍,对于另外两个残基,降低幅度为5至10倍。当将每个CTL/肽组合的相对抗原活性归一化为肽的相对竞争活性时,出现了一种显著的模式。对竞争活性影响最大的两个残基对识别没有超出竞争观察到的额外影响。与之形成鲜明对比的是,测试的其他五个位置的丙氨酸替代差异很大,这取决于CTL/肽组合。这种模式不仅支持了一种模型,即Tyr253和Ile260残基将肽锚定到Kd分子上,还意味着它们实际上无法被TCR识别。
