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首页> 外文期刊>Journal of Biochemical and Biophysical Methods >Small amounts of urea and guanidine hydrochloride can be detected by a far-UV spectrophotometric method in dialysed protein solutions.
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Small amounts of urea and guanidine hydrochloride can be detected by a far-UV spectrophotometric method in dialysed protein solutions.

机译:可以通过远紫外分光光度法在透析的蛋白质溶液中检测到少量的尿素和盐酸胍。

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摘要

The quantization of small amounts of chemical denaturants as urea or guanidine hydrochloride in protein solutions after dialysis is a difficult task in the molecular biology laboratory practice. Refractometric methods are useful to quantify a denaturant in the molar range but this methodology is not helpful when the denaturant is present in small amounts. The method herein described is a new comparative method that requires, a priori, the quantification of the stock solutions of urea (8 M) and guanidine hydrochloride (6 M) by refractometry to prepare by sequential dilution the standards used for comparison in the spectropolarimeter. The method is based on the observation that the wavelengths, at which the absorbance of polarized light increases in the far-UV region, as observed by spectropolarimetry, is related to the concentration of the chemical denaturant present in the protein solution. In the quantitation method herein reported, the urea and guanidine hydrochloride detection limits range from 1.2x10(-4) to 6x10(-6) M depending on the protein dialysis buffer used for a standard cell path length of 1 cm. The sensibility of this method results to be comprised in a range 4-5 orders of magnitude higher than that measured by refractometry. The determinations in both the sample and the control preparations are virtually completed within approximately 10 min.
机译:在分子生物学实验室实践中,透析后对蛋白质溶液中尿素或胍盐酸盐等少量化学变性剂进行定量是一项艰巨的任务。折光法可用于定量摩尔范围内的变性剂,但当变性剂少量存在时,此方法无用。本文所述的方法是一种新的比较方法,该方法事先需要通过折光法对尿素(8 M)和盐酸胍(6 M)的储备溶液进行定量,以通过顺序稀释来制备用于分光光度计中进行比较的标准品。该方法基于以下观察:通过分光旋光法观察到,在远紫外区域中偏振光的吸收率增加的波长与蛋白质溶液中存在的化学变性剂的浓度有关。在本文报道的定量方法中,取决于用于1 cm标准细胞路径长度的蛋白质透析缓冲液,尿素和胍盐酸盐的检测极限范围为1.2x10(-4)至6x10(-6)M。该方法的灵敏度比折光法测量的灵敏度高4-5个数量级。样品和对照制剂中的测定实际上在大约10分钟内完成。

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