Literature DB >> 18762158

Photocleavage-based affinity purification and printing of cell-free expressed proteins: application to proteome microarrays.

Mark Lim1, Kenneth J Rothschild.   

Abstract

Proteome microarrays hold great promise for various biotechnological and biomedical applications, including mapping protein-protein interactions, drug discovery, and biomarker discovery. However, the need to express, purify, and print thousands of functional proteins at high density on a microarray substrate presents challenges that limit their widespread availability and use. We report the development of new methods, based on photocleavage, for the purification and printing of nascent proteins. Photocleavable biotin (PC-biotin) is incorporated into nascent proteins by misaminoacylated transfer RNAs (tRNAs) used in a coupled transcription/translation rabbit reticulocyte cell-free expression system. Proteins were affinity isolated onto (strept)avidin-coated beads and then photoreleased (PC-SNAG). Compared with polyhistidine tag-based affinity purification, PC-SNAG provided a higher purity yet a comparable yield using a glutathione-S-transferase (GST) test protein. Antibody-mediated PC-SNAG is also demonstrated. PC-SNAG proteins were found to exhibit native enzymatic activity and were suitable for the printing of ordered protein microarrays used in protein-protein interaction assays. Alternatively, when beads carrying photocleavably tethered proteins were placed in close proximity to an activated planar surface and then illuminated, proteins were transferred directly to the surface (PC-PRINT) to form discrete spots whose dimensions match those of the beads. PC-PRINT can provide an inexpensive method to fabricate very large-scale, high-density proteome microarrays. Moreover, transferring the proteins off the beads significantly reduces background autofluorescence observed with common bead types. To decode nascent proteins that are deposited by PC-PRINT from individual beads, the feasibility of using photocleavable quantum dot codes is demonstrated.

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Year:  2008        PMID: 18762158      PMCID: PMC2784287          DOI: 10.1016/j.ab.2008.07.038

Source DB:  PubMed          Journal:  Anal Biochem        ISSN: 0003-2697            Impact factor:   3.365


  50 in total

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Journal:  Anal Biochem       Date:  2000-03-15       Impact factor: 3.365

2.  Printing proteins as microarrays for high-throughput function determination.

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3.  Photocleavable peptide-DNA conjugates: synthesis and applications to DNA analysis using MALDI-MS.

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Review 5.  tRNA-mediated protein engineering.

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8.  Cell-free expression and functional reconstitution of homo-oligomeric alpha7 nicotinic acetylcholine receptors into planar lipid bilayers.

Authors:  L K Lyford; R L Rosenberg
Journal:  J Biol Chem       Date:  1999-09-03       Impact factor: 5.157

9.  N-terminal labeling of proteins using initiator tRNA.

Authors:  Jerzy Olejnik; Sadanand Gite; Sergey Mamaev; Kenneth J Rothschild
Journal:  Methods       Date:  2005-07       Impact factor: 3.608

10.  The N-pentenoyl protecting group for aminoacyl-tRNAs.

Authors:  Michiel Lodder; Bixun Wang; Sidney M Hecht
Journal:  Methods       Date:  2005-07       Impact factor: 3.608

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  3 in total

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Journal:  Rapid Commun Mass Spectrom       Date:  2014-01-15       Impact factor: 2.419

Review 2.  Nanoscale Extracellular Vesicle Analysis in Alzheimer's Disease Diagnosis and Therapy.

Authors:  Pete Heinzelman; Tina Bilousova; Jesus Campagna; Varghese John
Journal:  Int J Alzheimers Dis       Date:  2016-04-26

3.  Photocleavage-based affinity purification of biomarkers from serum: Application to multiplex allergy testing.

Authors:  Zhi Wan; Heather P Ostendorff; Ziying Liu; Lynda C Schneider; Kenneth J Rothschild; Mark J Lim
Journal:  PLoS One       Date:  2018-02-01       Impact factor: 3.240

  3 in total

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