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使用 REVERT 总蛋白染色作为加载对照,在通过 Western blot 分析脑匀浆时,比使用管家蛋白具有显著优势:对代表不同性腺激素状态的样品进行分析。

Use of the REVERT total protein stain as a loading control demonstrates significant benefits over the use of housekeeping proteins when analyzing brain homogenates by Western blot: An analysis of samples representing different gonadal hormone states.

机构信息

University of Pittsburgh, Department of Pharmaceutical Sciences, 1004 Salk Hall, Pittsburgh, PA 15261, USA.

出版信息

Mol Cell Endocrinol. 2018 Sep 15;473:156-165. doi: 10.1016/j.mce.2018.01.015. Epub 2018 Feb 1.

Abstract

Western blot is routinely used to quantify differences in the levels of target proteins in tissues. Standard methods typically use measurements of housekeeping proteins to control for variations in loading and protein transfer. This is problematic, however, when housekeeping proteins also are affected by experimental conditions such as injury, disease, and/or gonadal hormone manipulations. Our goal was to evaluate an alternative and perhaps superior method for conducting Western blot analysis of brain tissue homogenates from rats with distinct physiologically relevant gonadal hormone states. Tissues were collected from the hippocampus, frontal cortex, and striatum of young adult female rats that either were ovariectomized to model surgical menopause, or were treated with the ovatotoxin 4-vinylcyclohexene diepoxide (VCD) to model transitional menopause. Tissues also were collected from rats with a normal estrous cycle killed at proestrus when estradiol levels are high, and at diestrus when estradiol levels are low. Western blot detection of α-tubulin, β-actin, and GAPDH was performed and were compared for sensitivity and reliability with a fluorescent total protein stain (REVERT). Results show that the total protein stain was much less variable across samples and had a greater linear range than α-tubulin, β-actin, or GAPDH. The stain was stable and easy to use, and did not interfere with the immunodetection or multiplexed detection of the housekeeping proteins. In addition, we show that normalization of our data to total protein, but not to GAPDH, revealed significant differences in α-tubulin expression in the hippocampus as a function of treatment, and that gel-to-gel consistency in measuring differences between paired samples run on multiple gels was significantly better when data were normalized to total protein than when normalized to GAPDH. These results demonstrate that the REVERT total protein stain can be used in Western blot analysis of brain tissue homogenates to control for variations in loading and protein transfer, and provides significant advantages over the use of housekeeping proteins for quantifying changes in the levels of multiple target proteins.

摘要

Western blot 通常用于定量组织中目标蛋白水平的差异。标准方法通常使用管家蛋白的测量来控制加载和蛋白转移的变化。然而,当管家蛋白也受到实验条件的影响,如损伤、疾病和/或性腺激素处理时,这就成了问题。我们的目标是评估一种替代方法,也许是一种更优越的方法,用于对具有不同生理相关性腺激素状态的大鼠脑组织匀浆进行 Western blot 分析。从年轻成年雌性大鼠的海马体、前额皮质和纹状体中收集组织,这些大鼠要么被卵巢切除术切除以模拟手术性绝经,要么用卵母细胞毒素 4-乙烯环己烯二环氧乙烷 (VCD) 处理以模拟过渡性绝经。还从处于发情周期的大鼠中收集组织,这些大鼠在发情前期(雌激素水平高时)和发情后期(雌激素水平低时)处死。进行 α-微管蛋白、β-肌动蛋白和 GAPDH 的 Western blot 检测,并与荧光总蛋白染色剂(REVERT)进行比较,以评估其敏感性和可靠性。结果表明,总蛋白染色剂在样品间的变化要小得多,线性范围也比 α-微管蛋白、β-肌动蛋白或 GAPDH 大。该染色剂稳定且易于使用,并且不会干扰管家蛋白的免疫检测或多重检测。此外,我们还表明,将数据归一化为总蛋白,而不是 GAPDH,可揭示α-微管蛋白表达在海马体中作为处理的函数的显著差异,并且在多个凝胶上运行的配对样品之间测量差异时,当数据归一化为总蛋白时,凝胶间一致性明显优于归一化为 GAPDH 时。这些结果表明,REVERT 总蛋白染色剂可用于 Western blot 分析脑组织匀浆,以控制加载和蛋白转移的变化,并为定量分析多个靶标蛋白水平的变化提供了比使用管家蛋白显著的优势。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/85ef/6045444/2205042dc22d/nihms938825f1.jpg

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