Literature DB >> 19892168

Quantitation of protein.

James E Noble1, Marc J A Bailey.   

Abstract

The measurement of protein concentration in an aqueous sample is an important assay in biochemistry research and development labs for applications ranging from enzymatic studies to providing data for biopharmaceutical lot release. Spectrophotometric protein quantitation assays are methods that use UV and visible spectroscopy to rapidly determine the concentration of protein, relative to a standard, or using an assigned extinction coefficient. Methods are described to provide information on how to analyze protein concentration using UV protein spectroscopy measurements, traditional dye-based absorbance measurements; BCA, Lowry, and Bradford assays and the fluorescent dye-based assays; amine derivatization and detergent partition assays. The observation that no single assay dominates the market is due to specific limitations of certain methods that investigators need to consider before selecting the most appropriate assay for their sample. Many of the dye-based assays have unique chemical mechanisms that are prone to interference from chemicals prevalent in many biological buffer preparations. A discussion of which assays are prone to interference and the selection of alternative methods is included.

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Year:  2009        PMID: 19892168     DOI: 10.1016/S0076-6879(09)63008-1

Source DB:  PubMed          Journal:  Methods Enzymol        ISSN: 0076-6879            Impact factor:   1.600


  80 in total

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3.  Selected Reaction Monitoring Mass Spectrometry for Absolute Protein Quantification.

Authors:  Nathan P Manes; Jessica M Mann; Aleksandra Nita-Lazar
Journal:  J Vis Exp       Date:  2015-08-17       Impact factor: 1.355

4.  The molecular mechanism of induction of unfolded protein response by Chlamydia.

Authors:  Zenas George; Yusuf Omosun; Anthony A Azenabor; Jason Goldstein; James Partin; Kahaliah Joseph; Debra Ellerson; Qing He; Francis Eko; Melissa A McDonald; Matthew Reed; Pavel Svoboda; Olga Stuchlik; Jan Pohl; Erika Lutter; Claudiu Bandea; Carolyn M Black; Joseph U Igietseme
Journal:  Biochem Biophys Res Commun       Date:  2018-11-28       Impact factor: 3.575

5.  The use of hydrogel microparticles to sequester and concentrate bacterial antigens in a urine test for Lyme disease.

Authors:  Temple A Douglas; Davide Tamburro; Claudia Fredolini; Benjamin H Espina; Benjamin S Lepene; Leopold Ilag; Virginia Espina; Emanuel F Petricoin; Lance A Liotta; Alessandra Luchini
Journal:  Biomaterials       Date:  2010-10-28       Impact factor: 12.479

6.  Machine learning reveals sex-specific 17β-estradiol-responsive expression patterns in white perch (Morone americana) plasma proteins.

Authors:  Justin Schilling; Angelito I Nepomuceno; Antonio Planchart; Jeffrey A Yoder; Robert M Kelly; David C Muddiman; Harry V Daniels; Naoshi Hiramatsu; Benjamin J Reading
Journal:  Proteomics       Date:  2015-06-11       Impact factor: 3.984

7.  A Periplasmic Complex of the Nitrite Reductase NirS, the Chaperone DnaK, and the Flagellum Protein FliC Is Essential for Flagellum Assembly and Motility in Pseudomonas aeruginosa.

Authors:  José Manuel Borrero-de Acuña; Gabriella Molinari; Manfred Rohde; Thorben Dammeyer; Josef Wissing; Lothar Jänsch; Sagrario Arias; Martina Jahn; Max Schobert; Kenneth N Timmis; Dieter Jahn
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8.  Glutathione S-transferase in northern freshwater fish: the effect of water mineralization.

Authors:  E V Borvinskaya; N N Nemova; L P Smirnov
Journal:  Dokl Biol Sci       Date:  2011-03-05

9.  Assessing and Improving Protein Sample Quality.

Authors:  Bertrand Raynal; Sébastien Brûlé; Stephan Uebel; Stefan H Knauer
Journal:  Methods Mol Biol       Date:  2021

10.  Rex (encoded by DVU_0916) in Desulfovibrio vulgaris Hildenborough is a repressor of sulfate adenylyl transferase and is regulated by NADH.

Authors:  G A Christensen; G M Zane; A E Kazakov; X Li; D A Rodionov; P S Novichkov; I Dubchak; A P Arkin; J D Wall
Journal:  J Bacteriol       Date:  2014-10-13       Impact factor: 3.490

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