An improved method for the heterologous production of soluble human ribosomal proteins in Escherichia coli

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作者
Danilo Correddu
José de Jesús Montaño López
Praveen G. Vadakkedath
Amy Lai
Jane I. Pernes
Paris R. Watson
Ivanhoe K. H. Leung
机构
[1] The University of Auckland,School of Chemical Sciences
[2] Universidad Nacional Autónoma de México,Facultad de Ingeniería
[3] Victoria University of Wellington,The MacDiarmid Institute for Advanced Materials and Nanotechnology
[4] University of Bristol,School of Cellular and Molecular Medicine
[5] Biomedical Sciences Building,School of Biological Sciences
[6] University Walk,Maurice Wilkins Centre for Molecular Biodiscovery
[7] Victoria University of Wellington,undefined
[8] The University of Auckland,undefined
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Human ribosomal proteins play important structural and functional roles in the ribosome and in protein synthesis. An efficient method to recombinantly produce and purify these proteins would enable their full characterisation. However, the production of human ribosomal proteins can be challenging. The only published method about the recombinant production of human ribosomal proteins involved the recovery of proteins from inclusion bodies, a process that is tedious and may lead to significant loss of yield. Herein, we explored the use of different Escherichia coli competent cells and fusion protein tags for the recombinant production of human ribosomal proteins. We found that, by using thioredoxin as a fusion protein, soluble ribosomal protein could be obtained directly from cell lysates, thus leading to an improved method to recombinantly produce these proteins.
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