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用于测定小组织样本中胸腺素β4的一步法及其通过高压液相色谱法与其他类胸腺素β4肽的分离。

One-step procedure for the determination of thymosin beta 4 in small tissue samples and its separation from other thymosin beta 4-like peptides by high-pressure liquid chromatography.

作者信息

Hannappel E

出版信息

Anal Biochem. 1986 Aug 1;156(2):390-6. doi: 10.1016/0003-2697(86)90270-8.

Abstract

Thymosin beta 4 has been determined by a simple and fast one-step procedure in different tissues of rats. The tissues (1 to 40 mg) were disintegrated and deproteinized by homogenization in perchloric acid. After neutralization by potassium hydroxide the supernatant solution was used for determining thymosin beta 4 by reverse-phase HPLC without further manipulations. Not only does this procedure avoid artificial proteolysis as effectively as extraction of tissues by guanidinium chloride or boiling buffer, but it offers two further advantages. First, no additional steps--as for example desalting--are necessary prior to HPLC and thus the risk of losing thymosin beta 4 is eliminated. Using this procedure thymosin beta 4 is recovered quantitatively. The method is linear over the range 0.04 to 1.13 nmol and thymosin beta 4 is well separated from other thymosin beta 4-like peptides known to be present in mammals; i.e., thymosin beta Ala4, thymosin beta 9, thymosin beta 10, and thymosin beta Arg10. Second, the acid-insoluble pellet of the same extract can be used to determine the DNA content of the sample. Thus it is possible to relate thymosin beta 4 to DNA, which then allows comparing cells of different tissues and cell lines to one another. This procedure is also applicable to small peptides soluble in perchloric acid.

摘要

胸腺素β4已通过一种简单快速的一步法在大鼠的不同组织中得以测定。将组织(1至40毫克)在高氯酸中匀浆以进行破碎和脱蛋白处理。用氢氧化钾中和后,上清液无需进一步处理即可用于通过反相高效液相色谱法测定胸腺素β4。该方法不仅能像用氯化胍或煮沸缓冲液提取组织那样有效地避免人为的蛋白水解,而且还具有另外两个优点。首先,在进行高效液相色谱分析之前无需额外步骤(例如脱盐),从而消除了胸腺素β4损失的风险。采用该方法可定量回收胸腺素β4。该方法在0.04至1.13纳摩尔范围内呈线性,且胸腺素β4与已知存在于哺乳动物中的其他类胸腺素β4肽(即胸腺素β丙氨酸4、胸腺素β9、胸腺素β10和胸腺素β精氨酸10)能很好地分离。其次,同一提取物的酸不溶性沉淀可用于测定样品的DNA含量。因此,可以将胸腺素β4与DNA关联起来,进而能够对不同组织的细胞和细胞系进行相互比较。该方法也适用于可溶于高氯酸的小肽。

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