Ortenzi C, Miceli C, Bradshaw R A, Luporini P
Department of Cell Biology, University of Camerino, Italy.
J Cell Biol. 1990 Aug;111(2):607-14. doi: 10.1083/jcb.111.2.607.
The polypeptide pheromone Er-1, purified from the ciliate Euplotes raikovi of mating type I and genotype mat-1/mat-1, was iodinated with 125I-Bolton-Hunter reagent to a sp act of 0.45-0.73 mu Ci/microgram of protein. This preparation of 125I-Er-1 bound specifically to high affinity binding sites on the same cells of mating type I. Binding of 125I-Er-1 occurred with an apparent Kd of 4.63 +/- 0.12 X 10(-9) M in cells in early stationary phase. It was estimated that these cells carry a total number of approximately 5 X 10(7) sites/cell, with a site density that falls in the range of 1,600-1,700/microns 2 of cell surface. Unlabeled Er-1, other homologous pheromones such as Er-2 and Er-10, antibodies specific for Er-1, and human IL-2 were shown to act as effective inhibitors of specific binding of 125I-Er-1 to mating type I cells. The "autocrine" nature of the identified specific high affinity binding sites for Er-1 was further substantiated by cross-linking experiments. These experiments revealed that mating type-I cell membranes contain one protein entity of Mr = 28,000 that is capable of reacting specifically with the homodimeric native form of Er-1.
从交配型I和基因型mat-1/mat-1的纤毛虫雷氏游仆虫中纯化得到的多肽信息素Er-1,用125I-博尔顿-亨特试剂进行碘化,比活度为0.45 - 0.73μCi/μg蛋白质。这种125I-Er-1制剂能特异性结合到交配型I相同细胞上的高亲和力结合位点。在早期稳定期细胞中,125I-Er-1的结合表观解离常数Kd为4.63±0.12×10(-9)M。据估计,这些细胞每个细胞总共带有约5×10(7)个位点,位点密度在细胞表面1600 - 1700/μm2范围内。未标记的Er-1、其他同源信息素如Er-2和Er-10、Er-1特异性抗体以及人白细胞介素-2均被证明是125I-Er-1与交配型I细胞特异性结合的有效抑制剂。通过交联实验进一步证实了所鉴定的Er-1特异性高亲和力结合位点的“自分泌”性质。这些实验表明,交配型I细胞膜含有一种分子量为28,000的蛋白质实体,它能够与Er-1的同源二聚体天然形式特异性反应。
