Immunoaffinity separation of plasma proteins by IgY microbeads: Meeting the needs of proteomic sample preparation and analysis

Immunoaffinity separation of plasma proteins by IgY microbeads: Meeting the needs of proteomic sample preparation and analysis

Separation of complex protein mixtures that have a wide dynamic range of concentration, such as plasma or serum, is a challenge for proteomic analysis. Sample preparation to remove high‐abundant proteins is essential for proteomics analysis. Immunoglobulin yolk (IgY) antibodies have unique and advan...

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Veröffentlicht in:Proteomics (Weinheim) 2005-08, Vol.5 (13), p.3314-3328
Hauptverfasser: Huang, Lei, Harvie, Gulia, Feitelson, Jerald S., Gramatikoff, Kosi, Herold, David A., Allen, David L., Amunngama, Ravi, Hagler, Rachel A., Pisano, Michael R., Zhang, Wei-Wei, Fang, Xiangming
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Albumins - chemistry
Animals
Biomarker
Biomarkers - chemistry
Blood Proteins - chemistry
Blood Proteins - isolation & purification
Chromatography, Liquid
Edetic Acid - chemistry
Electrophoresis, Gel, Two-Dimensional
Electrophoresis, Polyacrylamide Gel
Humans
Immunoglobulin yolk antibodies
Immunoglobulins - chemistry
Mass Spectrometry
Mice
Microspheres
Protein depletion
Protein separation
Proteomics - methods
Sample preparation
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container_end_page 3328
container_issue 13
container_start_page 3314
container_title Proteomics (Weinheim)
container_volume 5
creator Huang, Lei
Harvie, Gulia
Feitelson, Jerald S.
Gramatikoff, Kosi
Herold, David A.
Allen, David L.
Amunngama, Ravi
Hagler, Rachel A.
Pisano, Michael R.
Zhang, Wei-Wei
Fang, Xiangming
description Separation of complex protein mixtures that have a wide dynamic range of concentration, such as plasma or serum, is a challenge for proteomic analysis. Sample preparation to remove high‐abundant proteins is essential for proteomics analysis. Immunoglobulin yolk (IgY) antibodies have unique and advantageous features that enable specific protein removal to aid in the detection of low‐abundant proteins and biomarker discovery. This report describes the efficiency and effectiveness of IgY microbeads in separating 12 abundant proteins from plasma with an immunoaffinity spin column or LC column. The protein separation and sample preparation process was monitored via SDS‐PAGE, 2‐DE, LC‐MS/MS, or clinical protein assays. The data demonstrate the high specificity of the protein separation, with removal of 95–99.5% of the abundant proteins. IgY microbeads against human proteins can also selectively remove orthologous proteins of other mammals such as mouse, rat, etc. Besides the specificity and reproducibility of the IgY microbeads, the report discusses the factors that may cause potential variations in protein separation such as protein–protein interactions (known as “Interactome”), binding and washing conditions of immunoaffinity reagents, etc. A novel concept of Seppromics is introduced to address methodologies and science of protein separation in a context of proteomics.
doi_str_mv 10.1002/pmic.200401277
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source MEDLINE; Wiley Online Library All Journals
subjects Albumins - chemistry
Animals
Biomarker
Biomarkers - chemistry
Blood Proteins - chemistry
Blood Proteins - isolation & purification
Chromatography, Liquid
Edetic Acid - chemistry
Electrophoresis, Gel, Two-Dimensional
Electrophoresis, Polyacrylamide Gel
Humans
Immunoglobulin yolk antibodies
Immunoglobulins - chemistry
Mass Spectrometry
Mice
Microspheres
Protein depletion
Protein separation
Proteomics - methods
Sample preparation
title Immunoaffinity separation of plasma proteins by IgY microbeads: Meeting the needs of proteomic sample preparation and analysis
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