Proteome analysis of the triton-insoluble erythrocyte membrane skeleton

Avik Basu; Sandra Harper; Esther N Pesciotta; Kaye D Speicher; Abhijit Chakrabarti; David W Speicher

doi:10.1016/j.jprot.2015.08.004

Proteome analysis of the triton-insoluble erythrocyte membrane skeleton

J Proteomics. 2015 Oct 14:128:298-305. doi: 10.1016/j.jprot.2015.08.004. Epub 2015 Aug 10.

Authors

Avik Basu¹, Sandra Harper², Esther N Pesciotta³, Kaye D Speicher², Abhijit Chakrabarti⁴, David W Speicher⁵

Affiliations

¹ The Center for Systems and Computational Biology and Molecular and Cellular Oncogenesis Program, The Wistar Institute, Philadelphia, PA, USA; Crystallography and Molecular Biology Division, Saha Institute of Nuclear Physics, Kolkata, India.
² The Center for Systems and Computational Biology and Molecular and Cellular Oncogenesis Program, The Wistar Institute, Philadelphia, PA, USA.
³ The Center for Systems and Computational Biology and Molecular and Cellular Oncogenesis Program, The Wistar Institute, Philadelphia, PA, USA; Department of Pediatrics, Children's Hospital of Philadelphia, Philadelphia, PA, USA.
⁴ Crystallography and Molecular Biology Division, Saha Institute of Nuclear Physics, Kolkata, India.
⁵ The Center for Systems and Computational Biology and Molecular and Cellular Oncogenesis Program, The Wistar Institute, Philadelphia, PA, USA. Electronic address: speicher@wistar.org.

Abstract

Erythrocyte shape and membrane integrity is imparted by the membrane skeleton, which can be isolated as a Triton X-100 insoluble structure that retains the biconcave shape of intact erythrocytes, indicating isolation of essentially intact membrane skeletons. These erythrocyte "Triton Skeletons" have been studied morphologically and biochemically, but unbiased proteome analysis of this substructure of the membrane has not been reported. In this study, different extraction buffers and in-depth proteome analyses were used to more fully define the protein composition of this functionally critical macromolecular complex. As expected, the major, well-characterized membrane skeleton proteins and their associated membrane anchors were recovered in good yield. But surprisingly, a substantial number of additional proteins that are not considered in erythrocyte membrane skeleton models were recovered in high yields, including myosin-9, lipid raft proteins (stomatin, flotillin1 and 2), multiple chaperone proteins (HSPs, protein disulfide isomerase and calnexin), and several other proteins. These results show that the membrane skeleton is substantially more complex than previous biochemical studies indicated, and it apparently has localized regions with unique protein compositions and functions. This comprehensive catalog of the membrane skeleton should lead to new insights into erythrocyte membrane biology and pathogenic mutations that perturb membrane stability. Biological significance Current models of erythrocyte membranes describe fairly simple homogenous structures that are incomplete. Proteome analysis of the erythrocyte membrane skeleton shows that it is quite complex and includes a substantial number of proteins whose roles and locations in the membrane are not well defined. Further elucidation of interactions involving these proteins and definition of microdomains in the membrane that contain these proteins should yield novel insights into how the membrane skeleton produces the normal biconcave erythrocyte shape and how it is perturbed in pathological conditions that destabilize the membrane.

Keywords: Erythrocytes; Membrane composition; Membrane skeleton; Membrane structure; Proteomics; Triton Skeleton.

Publication types

Research Support, N.I.H., Extramural
Research Support, Non-U.S. Gov't

MeSH terms

Cells, Cultured
Erythrocyte Membrane / chemistry*
Humans
Membrane Microdomains / chemistry*
Membrane Proteins / chemistry*
Octoxynol / chemistry*
Proteome / analysis*
Proteome / chemistry*
Solubility

Substances

Membrane Proteins
Proteome
Octoxynol

Abstract

Publication types

MeSH terms

Substances

Grants and funding