Journal of Guangxi Normal University(Natural Science Edition) ›› 2017, Vol. 35 ›› Issue (2): 108-111.doi: 10.16088/j.issn.1001-6600.2017.02.016

Previous Articles     Next Articles

Reduced Light Intensity of Western Blot by Diluted Ultra-enhancedChemiluminescent Solution

FAN Caiwen, TANG Juan, LUO Qin, LI Lu, XIANG Qiu*   

  1. Science Experimental Center, Guilin Medical University, Guilin Guangxi 541004, China
  • Online:2017-07-25 Published:2018-07-25

PDF (PC)

162

Abstract: Based on specific binding of antigen and antibody, western blot analysis is used to detect a protein in complex samples. However, using conventional chemiluminescence detection, light of the protein band is weak and X film is not much exposed, and using ultra-enhanced chemiluminescence detection,light of the protein band is strong and X film is too much exposed, both development images of protein band are not ideal sometimes, when protein concentration of the samples is too low, especially when the protein to be detected is lower abundant in X film is samples. Therefore, the protein was detected with diluted ultra-enhanced chemiluminescent solution, and the protein band was clearly showed and the development image effect of protein bands was improved obviously, which indicates that the intensity of light emission could be reduced and the development image effect of the protein bands could be improved by dilution of ultra-enhanced chemiluminescent solution in western blot analysis.

Key words: western blot, ultra-enhanced chemiluminescent solution, chemiluminescence, dilution

CLC Number: 

  • R446.6
[1] 牟宏宇, 罗波, 何涛. Western blotting 中低丰度蛋白转膜方法改进[J]. 泸州医学院学报, 2014, 37(5):472-475.
[2] 张莉萍, 蒋纪恺, JOE T. Western-blot 检测蛋白表达的方法改进及初步应用[J]. 第三军医大学学报,2001,23(10):1242-1243.
[3] ZANGHERI M,DI N F,MIRASOLI M, et al. Chemiluminescence lateral flow immunoassay cartridge with integrated amorphous silicon photosensors array for human serum albumin detection in urine samples[J]. Analytical and Bioanalytical Chemistry,2016, 408(30):8869-8879.
[4] 高重天, 孙群. 如何正确估计蛋白质SDS聚丙烯酰胺凝胶电泳的样品加样量[J]. 生物学通报,2009,44(3):54.
[5] D’SOUZA A, SCOFIELD R H. Protein stains to detect antigen on membranes[J]. Methods in Molecular Bioloby,2009,536:433-440.
[6] LIU J, ZHANG L, FU C, et al. Employment of 4-(1,2,4-triazol-1-yl)phenol as a signal enhancer of the chemiluminescent luminol-H2O2-horseradish peroxidase reaction for detection of hepatitis C virus in real samples[J]. Luminescence, 2015, 30(8):1297-302.
[7] 张纪磊. 化学发光共振能量转移体系的研究及其在肿瘤标志物检测中的应用[D]. 青岛:青岛科技大学, 2011.
[1] WU Zhuoling. Comparative Study on Effects of Fixation Nuclear Membrane Proteins by Different Fixative Agents in Immunofluorescence [J]. Journal of Guangxi Normal University(Natural Science Edition), 2018, 36(1): 121-125.
[2] ZHUANG Fenghong, MA Jiangming, CHEN Liting,SU Jing, ZHANG Yajun, YU Fangming. The Physiological and Ecological Responses of Leaves ofIsoetes sinensis under Different pH Treatments [J]. Journal of Guangxi Normal University(Natural Science Edition), 2017, 35(2): 133-141.
[3] HUO Qun, LIU Jie, CHEN Li, LIAO Wei-jia. Influence of Cut-off Value of AFP on Diagnosis of Hepatic Cancer [J]. Journal of Guangxi Normal University(Natural Science Edition), 2014, 32(3): 121-124.
Viewed
Full text


Abstract

Cited
  Shared   
  Discussed   
No Suggested Reading articles found!
Copyright © Journal of Guangxi Normal University(Natural Science Edition), All Rights Reserved.
Tel: 0773-5857325 E-mail: gxsdzkb@mailbox.gxnu.edu.cn
Powered by Beijing Magtech Co. Ltd