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与正常受试者刺激分泌相关的无放射受体活性生长激素。

Radioreceptor-inactive growth hormone associated with stimulated secretion in normal subjects.

作者信息

Sneid D S, Jacobs L S, Weldon V V, Trivedi B L, Daughaday H

出版信息

J Clin Endocrinol Metab. 1975 Sep;41(3):471-4. doi: 10.1210/jcem-41-3-471.

Abstract

We have previously reported systematic discrepancies between radioreceptor (RRA) and radioimmunoassay (RIA) measurements of growth hormone (hGH) in acromegalic patients. Due to limitations in RRA sensitivity, such comparisons could not be made in normal subjects. RRA methodology has now been adapted to allow detection of hGH at normal circulating levels. Since variations in Na+, K+, Ca++, and Mg++, incubation at 37 C and 4 C, and delayed tracer addition failed to improve assay sensitivity, specimen size was increased to 300 mul and incubation volume to 1.5 ml, while holding the quantity of added receptor constant. Best assay sensitivity, in room temperature incubations in 25 mM Tris for 16 h at pH 7.6 and 10 mM Ca++, was 0.66 +/- 0.30 ng hGH per ml serum. Under these conditions, 200 mug hepatic receptor protein bount 15.8 +/- 0.83% of added 125I-hGH, and 8.72 +/- 0.85% of bound tracer was displaced by 0.25 ng added unlabeled hGH. Nonspecific depression of binding by serum did not impair assay sensitivity with most receptor preparations. The basal hGH measured by RIA (antiserum 68-416) in a group of normal short children was 1.97 ng/ml, similar to the RRA result, 1.89 ng/ml (P = NS). Comparative measurements were also made in selected samples of sufficient volume during the 1 1/2 h following administration of hGH secretagogues (insulin, arginine, L-dopa). In these samples, the RIA value was 9.34 +/- 0.68 and the RRA value 6.29 +/- 0.62 ng/ml (P less than 0.01); the RIA/RRA was 1.77 +/- 0.18. Thus, no significant measurement discrepancy was found in basal samples from normal subjects, in contrast to previous findings in acromegalics. The appearance of such a discrepancy within 90 min after stimulation of hGH might be due to RIA/RRA discordance in secreted molecular subspecies, or might arise from peripheral hGH metabolism.

摘要

我们之前曾报道过肢端肥大症患者生长激素(hGH)的放射受体测定法(RRA)与放射免疫测定法(RIA)测量结果之间存在系统性差异。由于RRA灵敏度的限制,无法在正常受试者中进行此类比较。现在已对RRA方法进行了改进,以能够检测正常循环水平的hGH。由于Na +、K +、Ca ++和Mg ++的变化、在37℃和4℃下孵育以及延迟加入示踪剂均未能提高测定灵敏度,因此将样本量增加至300μl,孵育体积增加至1.5ml,同时保持加入的受体量不变。在室温下于25mM Tris中、pH 7.6和10mM Ca ++条件下孵育16小时,最佳测定灵敏度为每毫升血清0.66±0.30ng hGH。在这些条件下,200μg肝受体蛋白结合了加入的125I - hGH的15.8±0.83%,加入0.25ng未标记的hGH可使8.72±0.85%的结合示踪剂被置换。血清对结合的非特异性抑制作用在大多数受体制剂中并未损害测定灵敏度。一组正常矮身材儿童通过RIA(抗血清68 - 416)测得的基础hGH为1.97ng/ml,与RRA结果1.89ng/ml相似(P = 无显著性差异)。在给予hGH促分泌素(胰岛素、精氨酸、左旋多巴)后的1个半小时内,还对选定的足够体积的样本进行了比较测量。在这些样本中,RIA值为9.34±0.68,RRA值为6.29±0.62ng/ml(P<0.01);RIA/RRA为1.77±0.18。因此,与之前在肢端肥大症患者中的发现相反,在正常受试者的基础样本中未发现显著的测量差异。hGH刺激后90分钟内出现这种差异可能是由于分泌的分子亚类中RIA/RRA不一致,或者可能源于外周hGH代谢。

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