Project description:In order to know the effect of the second messenger cyclic di-GMP (cdGMP) on the global transcription of A. baumannii AB0057, we performed a differential RNA sequencing (dRNA-seq) experiment comparing two AB0057 derivatives that allow IPTG-induced overexpression of the phosphodiesterase coding gene rocR (decreases cdGMP levels) or a constitutively active version of the diguanylate cyclase pleD (pleD*, increases cdGMP levels). As a result, 98 genes appeared upregulated >2-fold in high cdGMP conditions (overexpressing pleD*) whereas 143 were downregulated. In highlights, the gene functional groups showing the strongest transcriptional alterations were those related to biofilm formation (upregulated) and twitching motility (downregulated).

Project description:We perform RNA-seq for comparison of deleted cavA wiht empty vector and complemented strains in A. baumannii AB5075 in order to assess the transcription regulation uder the control of this cyclase. A. baumannii AB5075 ΔcavA EV and ΔcavA+cavA cultures were grown in LB medium with 1mM IPTG (3 biological replicates per strain) until reaching mid-exponential phase. At this point, cells were harvested, treated with RNAlate for preservation of total RNA and stored at -80 C. After that, total RNA was extracted from each sample. The results showed 234 differentially expressed genes of which 143 were upregulated and 91 were downregulated in the ΔcavA+cavA complemented strain compared to the deleted cavA mutant harbouring empty vector (ΔcavA EV). The gene functional groups showing the strongest transcriptional alterations were those related to twitching motility (upregulation of genes involves in biogenesis and control of Type IV pili and com genes) as well as biofilm formation, exopolysaccharides production and fimbriae biogenesis (downregulation of csu operon, pga operon and ABUW_2052-2055). Also, genes related to inter- and intracellular signalling were differentially expressed. Cyclic AMP response regulator vfr and genes involved in c-di-GMP synthesis (ABUW_2135) and degradation (ABUW_1138) were upregulated while another gene linked to c-di-GMP degradation (ABUW_2631) and autoinducer synthase encoding gene abaI (part of the quorum sensing signalling system) were downregulated.

Project description:We perform RNA-seq comparing a treatment with 1% saccharin to a mock treatment in A. baumannii AB5075 in order to describe the alterations in global transcription produced by this artificial sweetener. A. baumannii AB5075 cultures were grown in LB medium in the presence of 1% saccharin or a water control (3 biological replicates per condition) until reaching mid-exponential phase. At this point, cells were harvested, treated with RNAlate for preservation of total RNA and stored at -80 C. After that, total RNA was extracted from each sample. As a result, 165 genes appeared upregulated in the presence of saccharin, whereas 215 were downregulated. In highlights, the gene functional groups showing the strongest transcriptional alterations were those related to pili and frimbriae biogenesis, involved in biofilms formation, adhesion and twitching motility.

Project description:We perform RNA-seq comparing a treatment with 0.375 mM Kaempferol to a mock treatment (DMSO) in A. baumannii AB5075 in order to describe the alterations in global transcription produced by this phytochemical. A. baumannii AB5075 cultures were grown in LB medium in the presence of 0.375 mM Kaempferol or a DMSO control (3 biological replicates per condition) until reaching mid-exponential phase. At this point, cells were harvested, treated with RNAlater for preservation of total RNA and stored at -80 C. After that, total RNA was extracted from each sample. As a result, 99 genes appeared upregulated in the presence of Kaempferol whereas 18 were downregulated. In highlights, the gene functional groups showing the strongest transcriptional alterations were those related to iron acquisition, siderophore biosynthesis and iron transport genes.

Project description:We perform RNA-seq comparing a treatment with 1.33% acesulfame K to a mock treatment in A. baumannii AB5075 in order to describe the alterations in global transcription produced by this artificial sweetener. A. baumannii AB5075 cultures were grown in LB medium in the presence of 1.33% acesulfame K or a water control (3 biological replicates per condition) until reaching mid-exponential phase. At this point, cells were harvested, treated with RNAlate for preservation of total RNA and stored at -80 C. After that, total RNA was extracted from each sample. As a result, 212 genes appeared upregulated in the presence of acesulfame K, whereas 252 were downregulated. In highlights, the gene functional groups showing the strongest transcriptional alterations were those related to twtching motility and natural transformation (downregulation of genes involves in biogenesis and control of Type IV pili and com genes), as well as genes involved in iron acquisition and siderophore biosynthesis and an uncharacterised gene cluster that might be involved in detoxification of sulfonamide compounds.

Project description:The experiment contains native Tn-seq data for Acinetobacter baumannii strain AB5075 with different genetic alterations. The strain was grown at 37 degrees in LB medium and genomic DNA was isolated. We then used PCR to select for DNA regions containing a junction between ISAba13 and chromosomal DNA. Libraries were then prepared using these DNA fragments.

Project description:RNA-seq was used to compare the transcriptomes of wild type A. baumannii AB5075 and a spontaneously arising grey colony variant that carries a copy of the insertion sequence ISAba13 within the gtr52 gene.

Project description:Acinetobacter baumannii AB5075 Genome sequencing

Project description:We perform RNA-seq comparing A. baumannii AB5075 cells resuspended in water or diluted M9-succinate and desiccated during 24 h (relative humidity 8-12%) to cells resuspended in water before desiccation. A. baumannii AB5075 cultures (3 independent biological replicates) were grown overnight (approx. 16 h) in M9 minimal medium supplemented with Na-succinate 20 mM. Cultures were split in two and each half was washed 3 times either with distilled water or with M9-succinate 20 mM diluted 1:250 (v:v). OD600 of the cell supensions was adjusted to 1.0 and 1 ml from the water-suspended cells was withdrawn as a control comparison, washed with RNAlater and stored at -80 C until further processing. 1 ml of the OD-adjusted water- and M9-suspended cells were spotted on polystyrene Petri dishes and left to air-dry in a laminar flow hood. Once dried, the plates were placed in a chamber with Drierite until reaching a relative humidity of 8-12% and were incubated during 24 h. Finally, cells were harvested by directly resspending them in RNAlater and stored at -80 C. After that, total RNA was extracted from each sample and cDNA libraries were generated and sequenced. The different comparisons showed that: i) 309 and 279 genes were upregulated and downregulated, respectively, in cells ressupended in water and desiccated compared to the control; ii) 435 and 512 genes were upregulated and downregulated, respectively, in cells resuspended in diluted M9-succinate and desiccated compared to the control; iii) 327 and 242 genes were upregulated and downregulated, respectively, in the cells resupended in water and desiccated compared to the cells resuspended in diluted M9-succinate and desiccated.

Project description:The experiment contains 3C-seq data for Acinetobacter baumannii strain AB5075 with different genetic alterations. The strain was grown at 37 degrees in LB medium and nucleoprotein was cross-linked using formaldehyde. Genomic DNA was isolated and digested with NlaIII before being ligated with T4 ligase. Sequencing was then used to identify junctions between ligated DNA sequences.