Thus, the goal of this study was to investigate four different V. parahaemolyticus strain sets, each of distinct geographical ML323 supplier origin (a cold water population originating from the German North Sea and the Baltic Sea, two prawn associated strain sets originating from Sri Lanka and Ecuador and additionally seafood isolates from German retail) by using MLST analysis, in order to define sequence
polymorphism of the ATR inhibitor strains, investigate genetic polymorphisms and relationships among strains of the different regions and to analyze the probable evolutionary relationships among the strains. Therefore differences in the relationship of isolates in regard to sequence type, clonal complex and peptide sequence type affiliation 17DMAG were considered. To analyze peptide based differences a peptide-based MLST scheme was implemented into the pubMLST database. To obtain a more global overview previously available MLST data of isolates from other countries and continents were included. Methods Sampling of Vibrio parahaemolyticus isolates A total of 130 V. parahaemolyticus isolates from different geographical areas were analyzed. The strain set consisted of four groups based on the geographic origin of strains and the sampling events: the first group was obtained from prawn farms located in three Sri Lankan regions (n = 43) [30], the second group consists
of strains (n = 34) that were isolated from regional and imported food samples in Germany (at retail) of different geographic origins and sample types. Within
the third group 27 isolates obtained from local markets and prawn farms in Ecuador are grouped. Finally the fourth group consists of planktonic isolates from the North Sea, the Kattegat, the Skagerrak and the Baltic Sea (NB-Seas; n = 26). Additionally, the two Japanese clinical strains Carnitine palmitoyltransferase II V. parahaemolyticus ATCC 17802 and RIMD 2210633 served as reference strains for process control. Details on the individual strains are summarized in Additional file 1: Table S1. Rarefaction curves for the whole strain set, for the three geographical subsets as well as for the entire pubMLST dataset were calculated to evaluate if sampling was adequate and if the existing diversity was recorded [31]. Isolates were stored in Cryovials at –80°C (Cryobank; Mast Diagnostica, Bootle, UK). MLST analysis Prior to DNA analysis strains were grown overnight in alkaline peptone water (APW; 0.3% yeast extract, 1% peptone, 2% NaCl, pH 8; Merck, Darmstadt, Germany) at 37°C with shaking (200 rpm). Bacterial DNA was extracted using Chelex 100 Resin (BioRad, Hercules, USA) according to the manufacturer’s instructions. For MLST analysis, internal fragments of the genes dnaE, gyrB, recA, dtdS, pntA, pyrC and tnaA were amplified by PCR and sequenced using primers and protocols described on the V. parahaemolyticus MLST website [13, 14, 32]. Sequencing was performed in both directions.
No related posts.