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A rapid method for the large scale purification of the intermediate filament protein vimentin by single-stranded DNA-cellulose affinity chromatography
Authors:W.James Nelson  Constantin E. Vorgias  Peter Traub
Affiliation:Max-Planck-Institut für Zellbiologie Rosenhof, 6802 Ladenburg/Heidelberg, Germany
Abstract:A new method is described for the purification of the intermediate filament protein vimentin from Ehrlich ascites tumor cells using single-stranded DNA-cellulose affinity chromatography. The procedure is rapid and allows the large scale isolation of the protein. Partial characterization of vimentin shows that it has a molecular weight of 58000 and an apparent pI of 5.3. It can be degraded by the vimentin-specific, Ca2+-activated proteinase which results in the production of a characteristic set of degradation products. The vimentin also cross-reacts with the intermediate filament protein monoclonal antibody, α-IFA.
Keywords:ssDNA  single-stranded DNA  EAT  Ehrlich ascites tumor  IEF  isoelectric focusing
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