Literature DB >> 10194854

Inclusion body purification and protein refolding using microfiltration and size exclusion chromatography.

B Batas1, C Schiraldi, J B Chaudhuri.   

Abstract

The presence of inclusion body impurities can affect the refolding yield of recombinant proteins, thus there is a need to purify inclusion bodies prior to refolding. We have compared centrifugation and membrane filtration for the washing and recovery of inclusion bodies of recombinant hen egg white lysozyme (rHEWL). It was found that the most significant purification occurred during the removal of cell debris. Moderate improvements in purity were subsequently obtained by washing using EDTA, moderate urea solutions and Triton X-100. Centrifugation between each wash step gave a purer product with a higher rHEWL yield. With microfiltration, use of a 0.45 micron membrane gave higher solvent fluxes, purer inclusion bodies and greater protein yield as compared with a 0.1 micron membrane. Significant flux decline was observed for both membranes. Second, we studied the refolding of rHEWL. Refolding from an initial concentration of 1.5 mg ml-1, by 100-fold batch dilution gave a 43% recovery of specific activity. Purified inclusion bodies gave rise to higher refolding yields, and negligible activity was observed after refolding partially purified material. Refolding rHEWL with a size exclusion chromatography based process gave rise to a refolding yield of 35% that corresponded to a 20-fold dilution.

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Year:  1999        PMID: 10194854     DOI: 10.1016/s0168-1656(98)00197-7

Source DB:  PubMed          Journal:  J Biotechnol        ISSN: 0168-1656            Impact factor:   3.307


  12 in total

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7.  Strategies for the recovery of active proteins through refolding of bacterial inclusion body proteins.

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Review 9.  Wanted: more monitoring and control during inclusion body processing.

Authors:  Diana Humer; Oliver Spadiut
Journal:  World J Microbiol Biotechnol       Date:  2018-10-19       Impact factor: 3.312

10.  Identifying Ortholog Selective Fragment Molecules for Bacterial Glutaredoxins by NMR and Affinity Enhancement by Modification with an Acrylamide Warhead.

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Journal:  Molecules       Date:  2019-12-30       Impact factor: 4.411

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