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心房利钠因子的放射受体测定法。

Radioreceptor assay for atrial natriuretic factor.

作者信息

Gutkowska J, Carrier F, St-Louis J, Thibault G, Cantin M, Genest J

机构信息

Laboratory of Biochemistry of Hypertension, Clinical Research Institute of Montreal, Quebec, Canada.

出版信息

Anal Biochem. 1988 Jan;168(1):100-6. doi: 10.1016/0003-2697(88)90016-4.

Abstract

Interest in accurate measurement of atrial natriuretic factor (ANF) in biological fluids and various tissues has been stimulated by recent data indicating the possible role of ANF in the homeostasis of salt and water. The presence of high-affinity binding sites for ANF in rat glomeruli has allowed us to develop a rapid, sensitive, and simple radioreceptor assay (RRA). A saturable high-affinity binding site on the membranes of rat glomeruli has been characterized by a dissociation constant of 33 pM and binding capacity of 396 fmol/mg protein. Rat plasma extracts or atrial homogenates or standards were incubated with radioiodinated ANF and a preparation of rat glomerular membranes. The receptor-bound and free radioactivity were separated by filtration on Whatman GF/C paper after 1 h incubation at room temperature. The sensitivity of the RRA was 2.08 fmol. The effective concentration of standard ANF that displaced 50% of labeled receptor-bound ANF (EC50) was 43.3 +/- 2.6 fmol/ml (n = 7). Both intra- and interassay coefficients of variation were smaller than 11%. This RRA assay has been compared with radioimmunoassay (RIA). High correlations for 19 plasma extracts and 34 atrial homogenates (r = 0.973 and r = 0.954, respectively) tested by RRA and RIA were obtained. This good correlation between the two methods suggests that the immunoreactive material found in rat plasma and atrial homogenates also displays biological activity.

摘要

近期数据表明心房利钠因子(ANF)在盐和水平衡中可能发挥作用,这激发了人们对生物体液和各种组织中ANF进行精确测量的兴趣。大鼠肾小球中存在ANF的高亲和力结合位点,这使我们能够开发一种快速、灵敏且简单的放射受体分析方法(RRA)。大鼠肾小球膜上的一个可饱和高亲和力结合位点的解离常数为33 pM,结合容量为396 fmol/mg蛋白质。将大鼠血浆提取物、心房匀浆或标准品与放射性碘化ANF及大鼠肾小球膜制剂一起孵育。在室温下孵育1小时后,通过在Whatman GF/C滤纸上过滤来分离受体结合的和游离的放射性。RRA的灵敏度为2.08 fmol。使50%的标记受体结合ANF被置换的标准ANF的有效浓度(EC50)为43.3±2.6 fmol/ml(n = 7)。批内和批间变异系数均小于11%。已将这种RRA分析方法与放射免疫分析(RIA)进行了比较。通过RRA和RIA检测的19份血浆提取物和34份心房匀浆(分别为r = 0.973和r = 0.954)具有高度相关性。这两种方法之间的良好相关性表明,在大鼠血浆和心房匀浆中发现的免疫反应性物质也具有生物活性。

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