However when counting just confident protein identifications (two

However when counting just confident protein identifications (two or Dactolisib datasheet more peptide hits) this increase is less pronounced. Looking at confident protein identifications with PPS Silent®, the total number of outer membrane LOXO-101 manufacturer proteins increased from 38 to 42. However, PPS Silent® appears to enhance detection of non-membrane proteins over outer membrane proteins as the proportion of non-membrane proteins increased marginally, while the proportion of outer membrane proteins decreased in the samples

subjected to PPS Silent®. This suggests that outer membrane proteins are relatively resistant to solubilising in PPS Silent®, while non-membrane associated proteins solubilise more readily. When comparing the data generated from this study with previously published work by Coldham & Woodward, more OMPs (total of 54) were identified here in comparison to 34 reported in their study. However, there were proteins that were not identified by using the LPI™ FlowCell. Coldham & Woodward[20] identified 34 outer membrane proteins using a method based on fractionating the whole cell lysate into its various intracellular parts coupled with check details two dimensional HPLC-mass spectrometry (2D-LC-MS/MS). Of the 34 outer membrane proteins identified,

just over half (18) were found in our dataset. Overall there were 36 S. typhimurium OMPs identified in our dataset that were not reported previously [20] (Additional Methisazone file 2). Some of these differences may be due to the use of different strains and variation in microbial culture

conditions between both studies which will be reflected in their protein expression profiles. In addition, since the method used by Coldham & Woodward relied on multiple fractionation steps of the whole cell lysate, potential loss of outer membrane proteins, especially lower abundant ones could have occurred at each step in their workflow. Furthermore, it has been reported that results generated from mass spectrometry vary depending on the database search algorithm used to identify proteins [22]. The work carried out by Coldham &Woodward used the search algorithm SEQUEST, while in this study the search algorithm MASCOT was used. Therefore, the differences observed between the two methods could also be attributed to the database search algorithms and parameters used. Previous work carried out by Molloy et al [13] identified 30 outer membrane proteins from Escherichia coli (E. coli) which is closely related to S. Typhimurium using a method based on the enrichment of outer membrane proteins using sodium carbonate washes and incorporating the detergent ASB-14 to aid in solubilising them prior 2D GE. This study manages to identify 15 of the 30 outer membrane proteins. A further 15 outer membrane proteins reported by Molloy et al were not seen in this study while 39 outer membrane proteins were identified in this study that was not reported by Molloy et al.

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