COMPARISIONOFDIFFERENTPROTEINDETERMINATIONMETHODS
COMPARISION OF DIFFERENT PROTEIN DETERMINATION METHODSCompanyMethodDetection RangeApplications -CompatibilityAssay protocolPrecautions-InterferencesAbsorbance 280nm0.1-1 OD280nm/mlAbsorbance of aromatic amino-acids (Trp, Tyr and Phe at less extent). Only for purified proteins with known absorptivity factor (Use ExPASy ProtParam tool to inquire E1% 280nm)Read absorbance 280nm.Nucleic acid, de......阅读全文
COMPARISION-OF-DIFFERENT-PROTEIN-DETERMINATION-METHODS
COMPARISION OF DIFFERENT PROTEIN DETERMINATION METHODSCompanyMethodDetection RangeApplications -CompatibilityAssay protocolPrecautions-InterferencesA
Bradford-–-Protein-Determination
Bradford – Protein DeterminationIntroductionA rapid and accurate method for the estimation of protein concentration. The technique is simpler, faster
Lowry-–-Protein-Determination
Lowry – Protein Determination(From Protein Protocols on CD-ROM Humana Press, 1998 - Section 1-2 The Lowry Method for Protein Quantitation Jakob H. Wat
The-Determination-of-Proteinprotein-Interactions-by-the-Matingbased-...
Dynamic and reversible protein–protein interactions have a pivotal function in all living cells. For instance, protein–protein interactions are in
UV-Absorbance-(280-nm)--–-Protein-Determination
UV Absorbance (280 nm) – Protein Determination Simple and quick method to accurately quantitate total protein in purified material or approximately q
蛋白质定量分析(Protein-determination)
Bradford 的dye-binding method 是利用Coomassie brilliant blue G-250 (CBG) 可与蛋白质结合而变色的特性来定量 (Bradford, 1976);若试样中的蛋白质量较多,则结合到蛋白质而变色的CBG 也多,因而呈色较深。下例是以一组
蛋白质定量分析(Protein-determination)
实验概要本文介绍了蛋白质定量分析(Protein determination) Bradford 的dye-binding method的原理、样品配制及操作步骤等。实验原理Bradford 的dye-binding method 是利用Coomassie brilliant blue G-250
Different-types-of-human-cells
Human primary cells are cells taken from living human beings and cultured. These cells retain the differentiation of the original cells taken in
Protein-Crystallization
Background:Proteins, like many molecules, can be prompted to form crystals when placed in the appropriate conditions. In order to crystallize a protei
Methods-for-the-Measurement-of-a-Bacterial-Enzyme-Activity-in-Cell-Lysates3
Different enzyme assays for ACTase study in H. pyloriACTase properties were studied in situ in cell-free extracts to obtain information on enzyme func
蛋白质定量
Quantitative Determination of Peptides by Sulfhydryl (-SH) Groups New (Contributed by David Van Horn, Dept. of Chemistry, UC Berkeley Greg Bulaj, Dept
Comprehensive-identification-of-novel-proteins-and-Nglycosylation-sites四
Figure 2 Distribution of N-glycopeptides analyzed by different enriched methods and instruments of royal jelly proteins. A is the distribution of N-
分光光度计的使用
With the aid of spectroscopy, the quantitative analysis of nucleic acids and proteins has established itself as a routine method in many laboratories.
分光光度计知识
With the aid of spectroscopy, the quantitative analysis of nucleic acids and proteins has established itself as a routine method in many laboratories.
Quantification-made-easy
With the aid of spectroscopy, the quantitative analysis of nucleic acids and proteins has established itself as a routine method in many laboratories.
Determination-of-IC50
DescriptionIn vitro whole cell assay by [H3] Hypoxanthine uptake assay Procedure[H3] Hypoxanthine uptake assay (with respect to red blood cell culture
分子克隆蛋白表达实验指南(十二)
– Note: The yield of fusion protein can be estimated by measuring the absorbance at 280 nm. The GST affinity tag can be approximated by 1 A280 Å 0.5
Edman-Sequencing-of-Proteins-from-2D-Gels
The Western blotting/sequencing technique using polyvinylidene difluoride (PVDF) membrane is one of the most popular technique for Edman sequencin
采用生物信息学和实验方法联合分析转录组信息
The wealth of transcript information that has been made publicly available in recent years requires the development of high-throughput functional geno
Antibody-Purification-using-Protein-A,-Protein-G,-or-Protein-L-Agarose
实验概要This protocol is designed as a quick purification method for antibodies from mammalian sera, ascites, and cell culture supernatants. It should
Antibody-Purification-using-Protein-A,-Protein-G,-or-Protein-L-Agarose
实验概要This protocol is designed as a quick purification method for antibodies from mammalian sera, ascites, and cell culture supernatants主要试剂 Protein
抗体特异性检测提议问答国际抗体验证工作组
The International Working Group on Antibody Validation: 国际抗体验证工作组 Proposal for Antibody Specificity Testing Q&A 关于抗体特异性检测提议的常见问题及回答 1.What is th
Quantitative-Determination-of-Peptides-by-Sulfhydryl-(SH)-Groups
Quantitative Determination of Peptides by Sulfhydryl (-SH) GroupsAuthor: David Van Horn, Greg BulajSource: Contributed by David Van Horn, Dept. of Che
Cell-and-tissue-lysis-hub
This page should point you to the many different general and lab-specific protocols describing tissue and cell lysis and serve as forum for comparison
Twohybrid-analysis-of-genetic-regulatory-networks
1. Introduction and BackgroundThere is a great need for general methods to characterize the proteins that contemporary biology makes available. The li
Comprehensive-identification-of-novel-proteins-and-Nglycosylation-sites二
ResultsIdentified novel royal jelly proteins To expand the number of known proteins in the RJ proteome, RJ proteins were extracted and digested wit
ARID4B基因突变与药物因子介绍
该基因编码一种与视网膜母细胞瘤结合蛋白-1序列相似的蛋白质编码蛋白是组蛋白去乙酰化酶依赖的SIN3A转录辅压蛋白复合物的一个亚单位,在多种细胞过程中发挥作用,包括增殖、分化、凋亡、癌变和细胞命运的决定该基因产物被从乳腺癌患者中分离出来的IgG抗体识别,似乎是一种与多种人类恶性肿瘤相关的分子标记已鉴定
ARID4B基因编码功能及结构描述
该基因编码一种与视网膜母细胞瘤结合蛋白-1序列相似的蛋白质编码蛋白是组蛋白去乙酰化酶依赖的SIN3A转录辅压蛋白复合物的一个亚单位,在多种细胞过程中发挥作用,包括增殖、分化、凋亡、癌变和细胞命运的决定该基因产物被从乳腺癌患者中分离出来的IgG抗体识别,似乎是一种与多种人类恶性肿瘤相关的分子标记已鉴定
Determination-and-Detection-of-Reactive-Oxygen-Species-(ROS),-Lipid-...
Reactive oxygen species or intermediates are formed by the incomplete reduction of oxygen. Organisms living in aerobic environment generate variou
DNA-Immunoprecipitation-for-the-Determination-of-DNABinding-Specificity
Andrea J. Gossett and Jason D. Lieb1Department of Biology, University of North Carolina at Chapel Hill, Chapel Hill, NC 27599, USA1Corresponding autho