Yang C H, Sirotnak F M, Mines L S
Memorial Sloan-Kettering Cancer Center, New York, New York 10021.
J Biol Chem. 1988 Jul 15;263(20):9703-9.
Studies are reported on the characterization of a new isolate within a novel class of variants of the L1210 cell exhibiting markedly increased transport inward of folate analogues. This variant (L1210/R83), which was selected in the presence of the antifolate metoprine, exhibited a 40-fold increase in [3H]aminopterin influx compared to parental cells and a modest (4-5-fold) increase in [3H]aminopterin efflux. The increase in influx was associated with a comparable increase in influx Vmax for the one-carbon, reduced folate transport system and the same increase in the amount of specific binding of [3H]aminopterin on the cell surface. Values for influx Km for [3H]aminopterin and specificity for various folate structures were unchanged. The alteration in influx Vmax and more rapid efflux accounted for the different level of intracellular exchangeable level of drug at steady state in this variant compared with parental L1210 cells. Otherwise, membrane potential was unchanged. The N-hydroxysuccinimide ester of [3H]aminopterin was used to covalently label the specific binding protein for folate compounds in the plasma membrane of variant and parental L1210 cells. Incorporation of label into this protein was stable under a variety of conditions and accounted for 97 and 52% of total cellular labeling, respectively, for membrane derived from R83 and parental L1210 cells at a reagent concentration of 20 nM. Specific affinity labeling on the surface of parental and variant cells was decreased in the presence of aminopterin, methotrexate, or 5-formyltetrahydrofolate, but not in the presence of folic acid. Also, [3H]aminopterin influx in these cells was inhibited by the N-hydroxysuccinimide ester of aminopterin or methotrexate, but not the N-hydroxysuccinimide ester of folic acid. These findings, in addition to the increased affinity labeling of this variant, which corresponds to the increase in influx of [3H] aminopterin also seen, appears to identify the affinity labeled protein as a component of the "classical" one-carbon, reduced folate transport system in these cells. The affinity labeled protein from each cell type was solubilized in sodium dodecyl sulfate or extracted in detergent in the presence of proteinase inhibitors and was found to elute from Sephacryl S-300 and migrate during sodium dodecyl sulfate-polyacrylamide gel electrophoresis as a single peak of Mr = 45,000-48,000. Recovery of labeled binding protein in these fractions from R83 variant cells was approximately 40 times greater than that from parental cells.(ABSTRACT TRUNCATED AT 400 WORDS)
有研究报告了对L1210细胞新一类变体中一种新分离株的特性描述,该变体表现出叶酸类似物向内转运显著增加。这种变体(L1210/R83)是在抗叶酸药物美托普林存在的情况下筛选出来的,与亲代细胞相比,[3H]氨基蝶呤内流增加了40倍,[3H]氨基蝶呤外流适度增加(4 - 5倍)。内流增加与一碳、还原型叶酸转运系统的内流Vmax的相应增加以及[3H]氨基蝶呤在细胞表面特异性结合量的相同增加有关。[3H]氨基蝶呤的内流Km值和对各种叶酸结构的特异性未改变。内流Vmax的改变和更快的外流导致该变体与亲代L1210细胞在稳态时细胞内可交换药物水平不同。此外,膜电位未改变。[3H]氨基蝶呤的N - 羟基琥珀酰亚胺酯用于共价标记变体和亲代L1210细胞质膜中叶酸化合物的特异性结合蛋白。在各种条件下,标记掺入该蛋白是稳定的,在试剂浓度为20 nM时,分别占来自R83和亲代L1210细胞的膜总细胞标记的97%和52%。在氨基蝶呤、甲氨蝶呤或5 - 甲酰四氢叶酸存在下,亲代和变体细胞表面的特异性亲和标记降低,但在叶酸存在下未降低。此外,这些细胞中的[3H]氨基蝶呤内流受到氨基蝶呤或甲氨蝶呤的N - 羟基琥珀酰亚胺酯抑制,但不受叶酸的N - 羟基琥珀酰亚胺酯抑制。这些发现,除了该变体亲和标记增加外,这也与所见的[3H]氨基蝶呤内流增加相对应,似乎将亲和标记蛋白鉴定为这些细胞中“经典”一碳、还原型叶酸转运系统的一个组成部分。来自每种细胞类型的亲和标记蛋白在蛋白酶抑制剂存在下用十二烷基硫酸钠溶解或用去污剂提取,发现从Sephacryl S - 300洗脱并在十二烷基硫酸钠 - 聚丙烯酰胺凝胶电泳中迁移为Mr = 45,000 - 48,000的单峰。从R83变体细胞的这些级分中回收的标记结合蛋白比亲代细胞大约高40倍。(摘要截短至400字)
