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用于定量总蛋白的固相金属螯合分析法:对化学干扰的抗性

Solid-phase metal chelate assay for quantifying total protein: resistance to chemical interference.

作者信息

Lim M J, Patton W F, Shojaee N, Shepro D

机构信息

Boston University, MA, USA.

出版信息

Biotechniques. 1996 Nov;21(5):888-92, 894, 896-7. doi: 10.2144/96215rr01.

Abstract

Recently, we developed reversible metal chelate stains that are fully compatible with immunoblotting and protein sequencing. Membrane supports are incubated in Ferrozine/ferrous complex followed by ferrocyanide/ferric complex (double-metal chelate [DMC] stain). Proteins are quantified by computerized densitometry. In this study, the metal chelate stains are used for routine protein quantitation. Manually applying samples to membranes leads to variable spot spreading. Better results are achieved using a slot-blot apparatus to maintain a constant application area. The Ferrozine/ferrous and DMC assays are compared to colloidal gold and bicinchroninic acid (BCA) assays with respect to chemical interference, protein-to-protein variation, dynamic linear range and sensitivity. The DMC assay provides a superior linear range (100-fold range) and BCA assays (47-fold). Though the colloidal gold assay is more sensitive, it suffers from poor reproducibility, high protein-to-protein variation and lower tolerance to interfering agents. The BCA assay has the least protein-to-protein variation but is also least sensitive and most susceptible to interfering agents.

摘要

最近,我们开发了与免疫印迹和蛋白质测序完全兼容的可逆金属螯合染色剂。将膜支持物在亚铁嗪/亚铁络合物中孵育,然后在亚铁氰化物/铁络合物(双金属螯合 [DMC] 染色剂)中孵育。通过计算机密度测定法定量蛋白质。在本研究中,金属螯合染色剂用于常规蛋白质定量。手动将样品施加到膜上会导致斑点扩散不一致。使用狭缝印迹装置保持恒定的施加面积可获得更好的结果。就化学干扰、蛋白质间差异、动态线性范围和灵敏度而言,将亚铁嗪/亚铁和 DMC 测定法与胶体金和双辛可宁酸(BCA)测定法进行了比较。DMC 测定法提供了更优的线性范围(100 倍范围),BCA 测定法为 47 倍。虽然胶体金测定法更灵敏,但它的重现性差、蛋白质间差异大且对干扰剂的耐受性较低。BCA 测定法的蛋白质间差异最小,但也是最不灵敏且最易受干扰剂影响的。

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