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一种新建立的酶联免疫吸附测定法,用于显示雄性腺对四脊光壳螯虾血淋巴中次级卵黄发生特异性蛋白的影响。

A newly established ELISA showing the effect of the androgenic gland on secondary-vitellogenic-specific protein in the hemolymph of the crayfish Cherax quadricarinatus.

作者信息

Sagi A, Khalaila I, Abdu U, Shoukrun R, Weil S

机构信息

Department of Life Sciences, Ben-Gurion University of the Negev, Beer-Sheva, 84105, Israel.

出版信息

Gen Comp Endocrinol. 1999 Jul;115(1):37-45. doi: 10.1006/gcen.1999.7277.

Abstract

A quantitative enzyme-linked immunosorbent assay (ELISA) was developed to monitor the onset of secondary vitellogenesis in Cherax quadricarinatus females and in intersex individuals (having both male and female reproductive systems) after removal of the androgenic gland (AG). As a prerequisite for the assay, the 106-kDa polypeptide was separated from newly laid C. quadricarinatus eggs by SDS-PAGE, and anti-106-kDa antibody was raised in rabbit. The specificity of the anti-106-kDa polypeptide for proteins specific for the hemolymph of secondary-vitellogenic females was confirmed by double immunodiffusion and immunoblot cross-reactivity tests. A characteristic standard ELISA curve, using egg high-density lipoprotein (HDL), showed linearity between 16 and 500 ng (r = 0. 953) and was sensitive for amounts as low as 8 ng. The inter- and intraassay coefficients of variance were 14.8 and 7.2%, respectively. Only traces of egg HDL equivalents were detected in the hemolymph of male and primary-vitellogenic females (11 to 110 microg/ml), confirming the specificity of the assay, whereas high levels of such a protein (8-35 mg/ml) were detected in the hemolymph of secondary-vitellogenic females. Removal of the AG from intersex individuals leads to a significant increase in the concentration of vitellogenic-specific protein in the hemolymph (up to 2 mg/ml). Moreover, a significantly lower concentration was found in females subjected to AG transplant (79.3 microg/ml). The ELISA thus provided an accurate and sensitive tool to investigate the influence of the AG on the expression of a vitellogenic-specific protein in female and intersex C. quadricarinatus, confirming the central role of this gland in tuning sexual plasticity in this species.

摘要

开发了一种定量酶联免疫吸附测定(ELISA),用于监测四脊光壳蟹雌性个体和雌雄同体个体(具有雄性和雌性生殖系统)在摘除雄激素腺(AG)后二次卵黄发生的开始情况。作为该测定的前提条件,通过SDS-PAGE从新产下的四脊光壳蟹卵中分离出106-kDa多肽,并在兔体内产生抗106-kDa抗体。通过双向免疫扩散和免疫印迹交叉反应试验证实了抗106-kDa多肽对二次卵黄发生雌性个体血淋巴特异性蛋白质的特异性。使用卵高密度脂蛋白(HDL)的特征性标准ELISA曲线在16至500 ng之间呈线性(r = 0.953),对低至8 ng的量敏感。测定间和测定内变异系数分别为14.8%和7.2%。在雄性和初级卵黄发生雌性个体的血淋巴中仅检测到痕量的卵HDL等效物(11至110μg/ml),证实了该测定的特异性,而在二次卵黄发生雌性个体的血淋巴中检测到高水平的这种蛋白质(8 - 35 mg/ml)。从雌雄同体个体摘除AG会导致血淋巴中卵黄发生特异性蛋白质的浓度显著增加(高达2 mg/ml)。此外,在接受AG移植的雌性个体中发现浓度显著降低(79.3μg/ml)。因此,ELISA提供了一种准确且灵敏的工具,用于研究AG对四脊光壳蟹雌性和雌雄同体个体中卵黄发生特异性蛋白质表达的影响,证实了该腺体在调节该物种性别可塑性中的核心作用。

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