Site-specific C-terminal and internal loop labeling of proteins using sortase-mediated reactions

被引:0
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作者
Carla P Guimaraes
Martin D Witte
Christopher S Theile
Gunes Bozkurt
Lenka Kundrat
Annet E M Blom
Hidde L Ploegh
机构
[1] Whitehead Institute for Biomedical Research,Department of Biology
[2] Massachusetts Institute of Technology,undefined
[3] Present address: Bio-Organic Chemistry,undefined
[4] Stratingh Institute for Chemistry,undefined
[5] University of Groningen,undefined
[6] Groningen,undefined
[7] The Netherlands.,undefined
来源
Nature Protocols | 2013年 / 8卷
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摘要
Methods for site-specific modification of proteins should be quantitative and versatile with respect to the nature and size of the biological or chemical targets involved. They should require minimal modification of the target, and the underlying reactions should be completed in a reasonable amount of time under physiological conditions. Sortase-mediated transpeptidation reactions meet these criteria and are compatible with other labeling methods. Here we describe the expression and purification conditions for two sortase A enzymes that have different recognition sequences. We also provide a protocol that allows the functionalization of any given protein at its C terminus, or, for select proteins, at an internal site. The target protein is engineered with a sortase-recognition motif (LPXTG) at the place where modification is desired. Upon recognition, sortase cleaves the protein between the threonine and glycine residues, facilitating the attachment of an exogenously added oligoglycine peptide modified with the functional group of choice (e.g., fluorophore, biotin, protein or lipid). Expression and purification of sortase takes ∼3 d, and sortase-mediated reactions take only a few minutes, but reaction times can be extended to increase yields.
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页码:1787 / 1799
页数:12
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