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Titlebook: Basic Protein and Peptide Protocols; John M. Walker Book 1994 Humana Press 1994

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楼主: 军械
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Jan-Philipp Büchler,Christian Waltertein in a sample, such as total amino acid analysis, the Biuret reaction, and the Lowry method (. ref. .), but these do not allow quantification of one protein in a mixture of several. This may be done by chromatography and estimation of the content of the appropriate peak in the elution profile by
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Slavica Singer,Sunčica Oberman Peterkao elucidate the structure of the oligosaccharide moeities present. For further studies of the protein to be carried out it is essential that the amino acid peptide bonds remain intact during the release process, whereas this is not essential for further studies on the released oligosaccharides. Here
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Hidden Champions and Export Success effect of glycosylation on the function of the glycoprotein. However, to fully characterize the diversity of oligosaccharide structures within a glycoprotein it is necessary to assign each oligosaccharide structure to a particular glycosylation site (i.e., the site-specific glycosylation pattern).
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Austrian and Swiss Hidden Championsult of the experiment. Second, drying a gel that is fragile may make it easier to handle (say, during optical scanning or display on an overhead projector). Third, and most important, it may be necessary to dry a gel to allow the most efficient detection of radioactive samples on it by autoradiograp
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Basic Protein and Peptide Protocols978-1-59259-519-8Series ISSN 1064-3745 Series E-ISSN 1940-6029
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,Cultivating “No Bossing” Leadership, Bradford (.) has become the preferred method for quantifying protein in many laboratories. This technique is simpler, faster, and more sensitive than the Lowry method. Moreover, when compared with the Lowry method, it is subject to less interference by common reagents and nonprotein components of biological samples (..).
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