To date, a limited number of constantly expressed surface proteins have been described in M. agalactiae. selleckchem Among them, P30, P48, and P80 were described as antigens [19–21]; other proteins belong to the variable surface membrane proteins family (Vpma) [14, 17], and P40 was suggested to play an important role in attachment to the host cell [18]. Genetic approaches traditionally used for large scale investigation of protein sets have been poorly applied to
mycoplasmas. The expression of immunogenic Mycoplasma proteins in Escherichia coli expression libraries is hampered by the very high A+T content (almost 80%) and by the Mycoplasma-specific codon usage, resulting in abnormal internal transcription/translation check details and in premature termination, respectively [22, 23]. In 2007, the full genome sequence of the M. agalactiae type strain PG2 (PG2T) was published [24] and paved the way for systematic proteomic studies in mycoplasmas. The combination of 2-D PAGE and mass spectrometry (MS) is a well-established method for the systematic and comparative study of proteomes, since it allows the simultaneous visualization and identification of the protein complement of a cell. However, it is commonly reported that standard 2-D PAGE lacks in resolution of very hydrophobic and basic proteins,
which are particularly abundant in the Mycoplasma membrane [25–27]. Indeed, membrane proteins are poorly detected Methocarbamol in 2-D PAGE maps of Mycoplasma total protein extracts [22, 28]. Triton X-114 fractionation may assist in solving this problem, since it was demonstrated to SYN-117 in vivo enable a selective enrichment in hydrophobic proteins [29, 30]. Triton X-114 fractionation followed by 2-D PAGE remains the method of choice for proteomic characterization of the membrane protein
subset [31], and for differential analysis of membrane protein expression among bacterial strains [32]. More specifically, the recently developed Differential In Gel Electrophoresis (DIGE) [33–35], based on labeling of protein samples with fluorescent dyes before 2-D electrophoresis, enables the accurate analysis of differences in protein abundance between samples. However, considering the above mentioned intrinsic limitations of 2-D PAGE, other gel-based proteomic approaches, such as one-dimensional PAGE and Liquid Chromatography-Tandem Mass Spectrometry (GeLC-MS/MS) [36], can be combined with the 2-D PAGE/MS in order to mine deeper into a liposoluble proteome. In this study, the membrane proteome of M. agalactiae was characterized by means of Triton X-114 fractionation, 2-D PAGE-MS, GeLC-MS/MS, and Gene Ontology classification. Differential expression of membrane proteins among M. agalactiae strains was also evaluated by 2D DIGE. Results Extraction of bacterial proteins and isolation of liposoluble proteins This study was aimed to the systematic characterization of M. agalactiae PG2T membrane proteins by means of a gel-based proteomic approach.