Differential Proteome Analysis of the Preeclamptic Placenta Using Optimized Protein Extraction

Author:

Centlow Magnus1,Hansson Stefan R.1,Welinder Charlotte2

Affiliation:

1. Department of Obstetrics & Gynecology, Lund University, BMC C14, 221 84 Lund, Sweden

2. Department of Oncology, Lund University, Barngatan 2B, 221 85 Lund, Sweden

Abstract

The human placenta is a difficult tissue to work with using proteomic technology since it contains large amounts of lipids and glycogen. Both lipids and glycogen are known to interfere with the first step in the two-dimensional polyacrylamide gel electrophoresis (2D-PAGE), the isoelectric focusing. In order to gain the best possible protein separation on 2D-PAGE, an optimized sample preparation protocol for placental proteins was developed. Two different buffers, urea/CHAPS and Hepes, were used for solubilization in combination with six different precipitation methods. The removal of glycogen from the samples by centrifugation was crucial for the final proteome maps. Solubilization with urea/CHAPS in combination with dichloromethane/methanol or acidified acetone proved to be the best precipitation procedures. When applied to clinical placenta samples apolipoprotein A1 was found to be accumulated in the preeclamptic placenta, where it may either have a nutritional effect or act as a modifier of signal transduction.

Funder

Swedish Research Council

Publisher

Hindawi Limited

Subject

Health, Toxicology and Mutagenesis,Genetics,Molecular Biology,Molecular Medicine,General Medicine,Biotechnology

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