Among the up-regulated genes in the “translation” category included 50S ribosomal protein L1 (rplA), L20 (rplT), 30S ribosomal protein S2 (rpsB), and translation initiation factor IF-1 (infA) (Additional file 1). Since Ery targets 50S ribosomal proteins and block the ribosome elongation tunnel, this finding suggests that C. jejuni increases transcription of these genes in order to help recover the halted peptide elongation and resume translation as its immediate response against the antibiotic exposure. In the “Defense mechanism” category,
two genes were up-regulated after inhibitory treatment, which encode putative MATE family transport protein (cj0619) buy ARN-509 and ABC-type transmembrane transport protein (cj0607). The role of these genes in the adaptation to Ery treatment remains undetermined. The “cell motility” category comprised the largest proportion of up-regulated genes in response to an inhibitory dose of Ery in wild-type C. jejuni (Table 1), suggesting that enhanced motility might be Campylobacter’s initial escape response to this noxious stress. cj0061c, which encodes the σ28 transcription factor fliA and is essential for normal flagellar
biosynthesis [25], is up-regulated in NCTC 11168 when treated with inhibitory and sub-inhibitory doses of Ery (Table 3). This gene induction was independently confirmed by qRT-PCR (Table LGK-974 chemical structure 4). Previous research indicated that σ28 regulates the major flagellin gene (flaA) and other late genes of the flagellar regulon as well as some non-flagellar genes in C. jejuni[26]. Also, it has been demonstrated that the flaA promoter can be activated by the intestinal environment and C. jejuni chemotactic
effectors, such as bovine bile, deoxycholate, L-fucose, osmolarity, Adenosine aspartate, glutamate, organic acids citrate, fumarate, α-ketoglutarate and succinate [27]. The microarray and qRT-PCR results presented here revealed that Ery induced expression of this regulatory gene (fliA), which might explain why multiple motility genes were up-regulated in C. jejuni under Ery treatment. Compared with the inhibitory-dose Ery treatment, sub-inhibitory dose Ery triggered a much smaller response in the Torin 2 mouse overall transcription in C. jejuni (Table 2 and Additional file 1). There were no or limited changes in most COG categories, except for “poorly characterized” and “amino acid transport and metabolism”. For example, no differentially expressed genes were found in the “energy production and conversion” category under sub-inhibitory Ery treatment (Table 2), while a large portion of genes in this category were down-regulated under the treatment of an inhibitory does of Ery (Table 1).