Abstract

Protein purification is a vital and expensive step in biomedical research and in the development and manufacturing of therapeutic proteins. Unfortunately, affinity methods, which are at the heart of most protein purifications, often present a bottleneck in the separation process because of slow diffusion of proteins in the pores of chromatographic gels. Protein-absorbing membranes can overcome this challenge because convective flow through membrane pores provides rapid mass transport to binding sites. Such flow can also effectively remove undesired proteins to increase purity. However, membrane absorbers are not widely used for protein isolation because they have low protein-binding capacities.
The aim of this work is to modify membranes with functional polymer brushes to increase protein-binding capacities by an order of magnitude and enable rapid, selective protein purification. Additionally, properly designed brushes will be resistant to nonspecific adsorption and provide new methods for purification of """"""""sticky"""""""" proteins that are not amenable to column-based purification. This research will involve synthesis and characterization of polymer brush-modified membranes that bind histidine6- and glutathione S-transferrase-tagged proteins with minimal nonspecific adsorption. Preliminary results demonstrated purification of a histidine6-tagged protein in a cell extract, with a purity that greatly exceeds similar resin-based purification. Future work aims at developing brush-modified membranes in polymeric supports with pore sizes that will allow large increases in permeability. This will permit the use of lower pressures and thicker membranes with much higher capacities. Formation of such membranes will require both development of new synthetic methods that are compatible with polymer supports and growth of thicker brushes that rapidly bind more protein. Hence, protein binding and non-specific adsorption will be examined as a function of brush thickness, composition, density, and functionalization, and membrane composition and geometry. With new membranes in hand, a variety of tagged proteins expressed in E. coli will be purified including SNAP-50, human MIP synthase, and SNAPc complex. MIP synthase is vital for inositol biosynthesis, while SNAP proteins are critical in gene expression. Additionally, SNAP-50 provides an example of a sticky protein that cannot be purified with typical affinity gels.

Public Health Relevance

This research will yield rapid, inexpensive methods for isolating remarkably pure proteins. Such techniques will be crucial in production of therapeutic proteins as well as research studies aimed at isolating proteins to understand their structure and health- related function.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
3R01GM080511-02S1
Application #
7924257
Study Section
Biomaterials and Biointerfaces Study Section (BMBI)
Program Officer
Edmonds, Charles G
Project Start
2009-09-30
Project End
2011-08-31
Budget Start
2009-09-30
Budget End
2011-08-31
Support Year
2
Fiscal Year
2009
Total Cost
$174,303
Indirect Cost

  Institution

Name
Michigan State University
Department
Chemistry
Type
Schools of Arts and Sciences
DUNS #
193247145
City
East Lansing
State
MI
Country
United States
Zip Code
48824

  Publications

Saha, Sampa; Baker, Gregory L (2015) Substituent Effects in the Surface-Initiated ATRP of Substituted Styrenes. Appl Surf Sci 359:911-916
Wijeratne, Salinda; Bruening, Merlin L; Baker, Gregory L (2013) Layer-by-layer assembly of thick, Cu(2+)-chelating films. Langmuir 29:12720-9
Tan, Yu-Jing; Sui, Dexin; Wang, Wei-Han et al. (2013) Phosphopeptide enrichment with TiO2-modified membranes and investigation of tau protein phosphorylation. Anal Chem 85:5699-706
Ma, Yiding; Dong, Jinlan; Bhattacharjee, Somnath et al. (2013) Increased protein sorption in poly(acrylic acid)-containing films through incorporation of comb-like polymers and film adsorption at low pH and high ionic strength. Langmuir 29:2946-54
Anuraj, Nishotha; Bhattacharjee, Somnath; Geiger, James H et al. (2012) An all-aqueous route to polymer brush-modified membranes with remarkable permeabilites and protein capture rates. J Memb Sci 389:117-125
Saha, Sampa; Bruening, Merlin L; Baker, Gregory L (2012) Surface-initiated Polymerization of Azidopropyl Methacrylate and its Film Elaboration via Click Chemistry. Macromolecules 45:
Tan, Yu-Jing; Wang, Wei-Han; Zheng, Yi et al. (2012) Limited proteolysis via millisecond digestions in protease-modified membranes. Anal Chem 84:8357-63
Bhattacharjee, Somnath; Dong, Jinlan; Ma, Yiding et al. (2012) Formation of high-capacity protein-adsorbing membranes through simple adsorption of poly(acrylic acid)-containing films at low pH. Langmuir 28:6885-92
Saha, Sampa; Bruening, Merlin L; Baker, Gregory L (2011) Facile synthesis of thick films of poly(methyl methacrylate), poly(styrene), and poly(vinyl pyridine) from Au surfaces. ACS Appl Mater Interfaces 3:3042-8
Wang, Wei-Han; Dong, Jin-Lan; Baker, Gregory L et al. (2011) Bifunctional polymer brushes for low-bias enrichment of mono- and multi-phosphorylated peptides prior to mass spectrometry analysis. Analyst 136:3595-8

Showing the most recent 10 out of 15 publications