首页 | 本学科首页   官方微博 | 高级检索  
     


A sensitive fluorometric assay for quantitatively measuring specific peptide binding to HLA class I and class II molecules
Authors:Tom H. M. Ottenhoff   Annemieke Geluk   Mireille Toebes   Willemien E. Benckhuijsen   Krista E. van Meijgaarden  Jan Wouter Drijfhout
Affiliation:

Department of Immunohematology and Blood Bank, Leiden University Hospital, Leiden, Netherlands

Abstract:
A sensitive, highly reproducible assay was developed for measuring binding of peptides to various HLA class I and II alleles. The assay is based on competition for binding to HLA between a peptide of interest and a fluorescent labelled standard peptide. This mixture is incubated with HLA to obtain equilibrium binding, and subsequently separated on an HPLC size-exclusion column in (i) a protein fraction containing HLA and bound peptide and (ii) a free peptide fraction. Each assay uses only 100 fmol labelled peptide and approximately 10 pmol of HLA. The analytical system contains an autosampler that samples from 96-well microtiter plates. Injections and data recording/evaluation is fully automated. Typical analysis time is 10–12 min per sample. The fluorescence in the HLA-bound peptide and free peptide containing fractions is measured on-line. The ratios of fluorescence signal in protein and peptide fractions at various concentrations of the peptide of interest are determined. IC50 values are calculated from the binding curve as obtained by curve fitting of the data. Here we show results for peptide binding to HLA-DR1 and -DR17 molecules purified from detergent solubilized cell lysates, and for recombinant HLA-A* 0201 and HLA-A* 0301 expressed in E. coli.

The assay reported is sensitive and reproducible. It is non-radioactive and is non-labor intensive due to the high degree of automation.

Keywords:Fluorometric assay   Peptide binding   HLA class I   HLA class II
本文献已被 ScienceDirect 等数据库收录!
设为首页 | 免责声明 | 关于勤云 | 加入收藏

Copyright©北京勤云科技发展有限公司  京ICP备09084417号