Differential proteomic screening and identification for non-traumatic necrotic femoral osseous tissue

Peng Yan; Yeping Zhu; Hui Zhao; Yanyan Lu; Yuzhong Gao

doi:10.3892/etm.2017.4326

Differential proteomic screening and identification for non-traumatic necrotic femoral osseous tissue

Exp Ther Med. 2017 Jun;13(6):2900-2904. doi: 10.3892/etm.2017.4326. Epub 2017 Apr 12.

Authors

Peng Yan¹, Yeping Zhu², Hui Zhao¹, Yanyan Lu¹, Yuzhong Gao¹

Affiliations

¹ Department of Orthopedics, The First Affiliated Hospital of Jinzhou Medical University, Jinzhou, Liaoning 121000, P.R. China.
² Recovery Unit, Jinzhou Central Hospital, Jinzhou, Liaoning 121000, P.R. China.

Abstract

Currently, there is a lack of effective early screening and detection methods for femoral head necrosis. Current research on most orthopedic diseases focuses on proteomics in the preliminary stage. The recent fluorescence differential in gel electrophoresis (DIGE) has advantages such as a high reproducibility, high sensitivity, high throughput, and high dynamic range. It is currently one of the most widely used quantitative proteomic research means. We conducted this study to investigate the pathogenesis of non-traumatic femoral head necrosis using the fluorescence DIGE to screen non-traumatic femoral head necrosis based on proteomics and provide a theoretical basis for screening possible biomarkers and molecular targeted treatment. The DIGE technique was used to separate the protein. An electrophoretogram was established on the basis of scanning and analysis. Identification and a bioinformatics analysis were conducted for the differential protein. The protein with differential expression of over 2-fold was excavated and ionized by means of substrate assisted laser desorption. The flight time was identified with a mass spectrometer (matrix-assisted laser desorption/ionization time-of-flight mass spectrometry, MALDI-TOF/TOF). The formation on sequences, structures and functions of these proteins were obtained through database retrieval. Western blot analysis was used to verify the differential protein expression and the reliability of the DIGE result was verified. DIGE was used to successfully separate 1,500±40 protein spots. There were 252 significant differential protein spots. The Ettan™ Spot Picker automatic work station was used to excavate 49 significant differential protein spots with expression difference over 2-fold. The MALDI-TOF/TOF mass spectrometer was used to identify these differential protein spots. Six proteins were identified in total, which include apolipoprotein A1 (APOA1), fibrous protein original chain, fibrous protein original chain, serum albumin, sulfur-oxygen protein peroxiredoxin 2 (PRDX2) and actin. APOA1 and PRDX2 were subject to western blot analysis detection; results were consistent with the DIGE result. Based on an analysis of the biological information, these proteins may be associated with the incidence and progression of femoral head necrosis.

Keywords: bioinformatics; femoral head necrosis; fluorescence differential gel electrophoresis; mass spectrum; proteomics.