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通过高效离子交换色谱法分析雌激素受体的异构体

Isoforms of estrogen receptors by high-performance ion-exchange chromatography.

作者信息

Wiehle R D, Wittliff J L

出版信息

J Chromatogr. 1984 Aug 3;297:313-26. doi: 10.1016/s0021-9673(01)89051-8.

DOI:10.1016/s0021-9673(01)89051-8
PMID:6490763
Abstract

SynChropak AX-300, AX-500 and AX-1000 columns were used to separate ionic forms of estrogen receptors by high-performance ion-exchange chromatography. Cytosols from hormone-responsive tissues were incubated for 4-10 h with 3-4 nM [16 alpha-125I]iodoestradiol-17 beta, cleared of unbound ligand and applied to an anion-exchange column. Components were eluted at pH 7.4 using a gradient of phosphate buffer at 4-6 degrees C. Non-specific binding components were identified by chromatographing, the identical cytosol, incubated with [125I]iodoestradiol and a 500-fold excess of diethylstilbestrol, which blocks specific binding sites. [125I]Iodoestradiol was applied to the column in the absence of cytosol and eluted normally to determine the behavior of free ligand. Each column exhibited a different elution pattern for the estrogen receptor. The various isoforms of estrogen receptor were eluted differently from each column usually in the 15-120 mM and 180-250 mM region of the gradient. Often one non-specific binding component was not retained whereas other non-specific species were retained and eluted from the column in a salt-dependent manner; their position in the gradient varied from column to column. Similarly, free [125I]iodoestradiol was eluted at different positions in the gradients, dependent upon which column was employed. In general, the high flow-rates, reproducibility, good recovery and the apparent differential selectivity of each of the columns appear valuable in the investigation of the nature and subunit composition of the estrogen receptor molecule.

摘要

使用SynChropak AX - 300、AX - 500和AX - 1000色谱柱,通过高效离子交换色谱法分离雌激素受体的离子形式。将来自激素反应性组织的胞质溶胶与3 - 4 nM [16α - 125I]碘雌二醇 - 17β孵育4 - 10小时,去除未结合的配体后应用于阴离子交换柱。在4 - 6℃下,使用磷酸盐缓冲液梯度在pH 7.4条件下洗脱各组分。通过对相同的胞质溶胶进行色谱分析来鉴定非特异性结合组分,该胞质溶胶与[125I]碘雌二醇和500倍过量的己烯雌酚孵育,己烯雌酚可阻断特异性结合位点。在没有胞质溶胶的情况下将[125I]碘雌二醇应用于柱中并正常洗脱,以确定游离配体的行为。每种色谱柱对雌激素受体呈现出不同的洗脱模式。雌激素受体的各种同工型通常在梯度的15 - 120 mM和180 - 250 mM区域从各色谱柱中以不同方式洗脱。通常一种非特异性结合组分不被保留,而其他非特异性物质被保留并以盐依赖的方式从柱中洗脱;它们在梯度中的位置因柱而异。同样,游离的[125I]碘雌二醇在梯度中的洗脱位置也不同,这取决于所使用的色谱柱。一般来说,各色谱柱的高流速、重现性、良好的回收率以及明显的差异选择性在研究雌激素受体分子的性质和亚基组成方面似乎很有价值。

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