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Suppression of isotope scrambling in cell-free protein synthesis by broadband inhibition of PLP enzymes for selective 15 N-labelling and production of perdeuterated proteins in H 2 O

Su, Xun-Cheng; Loh, Choy; Qi, Ruhu; Otting, Gottfried

Description

Selectively isotope labelled protein samples can be prepared in vivo or in vitro from selectively labeled amino acids but, in many cases, metabolic conversions between different amino acids result in isotope scrambling. The best results are obtained by cell-free protein synthesis, where metabolic enzymes are generally less active, but isotope scrambling can never be suppressed completely. We show that reduction of E. coli S30 extracts with NaBH4 presents a simple and inexpensive way to achieve...[Show more]

dc.contributor.authorSu, Xun-Cheng
dc.contributor.authorLoh, Choy
dc.contributor.authorQi, Ruhu
dc.contributor.authorOtting, Gottfried
dc.date.accessioned2015-12-10T23:26:10Z
dc.identifier.issn0925-2738
dc.identifier.urihttp://hdl.handle.net/1885/67647
dc.description.abstractSelectively isotope labelled protein samples can be prepared in vivo or in vitro from selectively labeled amino acids but, in many cases, metabolic conversions between different amino acids result in isotope scrambling. The best results are obtained by cell-free protein synthesis, where metabolic enzymes are generally less active, but isotope scrambling can never be suppressed completely. We show that reduction of E. coli S30 extracts with NaBH4 presents a simple and inexpensive way to achieve cleaner selective isotope labelling in cell-free protein synthesis reactions. The purpose of the NaBH4 is to inactivate all pyridoxal-phosphate (PLP) dependent enzymes by irreversible reduction of the Schiff bases formed between PLP and lysine side chains of the enzymes or amino groups of free amino acids. The reduced S30 extracts retain their activity of protein synthesis, can be stored as well as conventional S30 extracts and effectively suppress conversions between different amino acids. In addition, inactivation of PLP-dependent enzymes greatly stabilizes hydrogens bound to α-carbons against exchange with water, minimizing the loss of α-deuterons during cell-free production of proteins from perdeuterated amino acids in H2O solution. This allows the production of highly perdeuterated proteins that contain protons at all exchangeable positions, without having to back-exchange labile deuterons for protons as required for proteins that have been synthesized in D2O.
dc.publisherKluwer Academic Publishers
dc.sourceJournal of Biomolecular NMR
dc.subjectKeywords: amino acid; deuterium oxide; isotope; nitrogen 15; pyridoxal 5 phosphate; Schiff base; sodium borohydride; article; cell free system; enzyme inactivation; enzyme inhibition; Escherichia coli; hydrogen bond; isotope labeling; nonhuman; priority journal; pr Cell-free protein synthesis; Isotope scrambling; NaBH 4; Pyridoxal phosphate; Selective 15N labeling
dc.titleSuppression of isotope scrambling in cell-free protein synthesis by broadband inhibition of PLP enzymes for selective 15 N-labelling and production of perdeuterated proteins in H 2 O
dc.typeJournal article
local.description.notesImported from ARIES
local.identifier.citationvolume50
dc.date.issued2011
local.identifier.absfor030606 - Structural Chemistry and Spectroscopy
local.identifier.absfor060107 - Enzymes
local.identifier.ariespublicationf2965xPUB1493
local.type.statusPublished Version
local.contributor.affiliationSu, Xun-Cheng, College of Physical and Mathematical Sciences, ANU
local.contributor.affiliationLoh, Choy, College of Physical and Mathematical Sciences, ANU
local.contributor.affiliationQi, Ruhu, College of Physical and Mathematical Sciences, ANU
local.contributor.affiliationOtting, Gottfried, College of Physical and Mathematical Sciences, ANU
local.description.embargo2037-12-31
local.bibliographicCitation.issue1
local.bibliographicCitation.startpage35
local.bibliographicCitation.lastpage42
local.identifier.doi10.1007/s10858-011-9477-5
local.identifier.absseo970106 - Expanding Knowledge in the Biological Sciences
dc.date.updated2016-02-24T08:14:33Z
local.identifier.scopusID2-s2.0-80051665061
local.identifier.thomsonID000290044400004
CollectionsANU Research Publications

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