BACKGROUND:Chromium is a toxic heavy metal, which primarily exists in two inorganic forms, Cr(VI) and Cr(III). Chromate Cr(VI)] is carcinogenic, mutational, and teratogenic due to its strong oxidizing nature. Biotransformation of Cr(VI) to less-toxic Cr(III) by chromate-resistant and reducing bacteria has offered an ecological and economical option for chromate detoxification and bioremediation. However, knowledge of the genetic determinants for chromate resistance and reduction has been limited so far. Our main aim was to investigate chromate resistance and reduction by Bacillus cereus SJ1, and to further study the underlying mechanisms at the molecular level using the obtained genome sequence.RESULTS:Bacillus cereus SJ1 isolated from chromium-contaminated wastewater of a metal electroplating factory displayed high Cr(VI) resistance with a minimal inhibitory concentration (MIC) of 30 mM when induced with Cr(VI). A complete bacterial reduction of 1 mM Cr(VI) was achieved within 57 h. By genome sequence analysis, a putative chromate transport operon, chrIA1, and two additional chrA genes encoding putative chromate transporters that likely confer chromate resistance were identified. Furthermore, we also found an azoreductase gene azoR and four nitroreductase genes nitR possibly involved in chromate reduction. Using reverse transcription PCR (RT-PCR) technology, it was shown that expression of adjacent genes chrA1 and chrI was induced in response to Cr(VI) but expression of the other two chromate transporter genes chrA2 and chrA3 was constitutive. In contrast, chromate reduction was constitutive in both phenotypic and gene expression analyses. The presence of a resolvase gene upstream of chrIA1, an arsenic resistance operon and a gene encoding Tn7-like transposition proteins ABBCCCD downstream of chrIA1 in B. cereus SJ1 implied the possibility of recent horizontal gene transfer.CONCLUSION:Our results indicate that expression of the chromate transporter gene chrA1 was inducible by Cr(VI) and most likely regulated by the putative transcriptional regulator ChrI. The bacterial Cr(VI)-resistant level was also inducible. The presence of an adjacent arsenic resistance gene cluster nearby the chrIA1 suggested that strong selective pressure by chromium and arsenic could cause bacterial horizontal gene transfer. Such events may favor the survival and increase the resistance level of B. cereus SJ1.
展开▼
机译:背景:铬是一种有毒的重金属,主要以两种无机形式存在,即六价铬和三价铬。铬酸盐Cr(VI)]具有强氧化性,因此具有致癌性,突变性和致畸性。通过抗铬酸盐和还原细菌将六价铬生物转化为毒性较低的三价铬,为铬酸盐的解毒和生物修复提供了一种生态和经济的选择。但是,到目前为止,关于铬酸盐抗性和还原性的遗传决定因素的知识是有限的。我们的主要目的是研究蜡状芽孢杆菌SJ1对铬的抗性和还原能力,并使用获得的基因组序列在分子水平上进一步研究其潜在机制。结果:从金属电镀厂的铬污染废水中分离出的蜡状芽孢杆菌SJ1显示出较高的Cr(VI)耐药性,当用Cr(VI)诱导时的最小抑制浓度(MIC)为30 mM。在57小时内,细菌完全减少了1 mM Cr(VI)。通过基因组序列分析,鉴定出假定的铬酸盐转运操纵子chrIA1和另外两个编码假定的铬酸盐转运蛋白的chrA基因,这些基因可能赋予铬酸盐抗性。此外,我们还发现了一个偶氮还原酶基因azoR和四个硝基还原酶基因nitR可能与铬酸盐的还原有关。使用逆转录PCR(RT-PCR)技术,表明邻近的基因chrA1和chrI的表达被诱导响应Cr(VI),但其他两个铬酸盐转运蛋白基因chrA2和chrA3的表达是组成型的。相反,在表型和基因表达分析中,铬酸盐还原是组成性的。结论:在蜡状芽孢杆菌SJ1中,chrIA1上游有一个resolvase基因,一个砷抗性操纵子和一个编码ChrIA1下游的Tn7样转座蛋白ABBCCCD的基因,暗示了近期水平基因转移的可能性。结论:我们的结果表明铬转运蛋白基因chrA1是由Cr(VI)诱导的,最有可能受推定的转录调节子ChrI调控。细菌对Cr(VI)的抗性水平也是可诱导的。在chrIA1附近存在一个相邻的抗砷抗性基因簇,这表明铬和砷的强选择压力可能导致细菌水平基因转移。这样的事件可能有利于蜡状芽孢杆菌SJ1的存活并增加其抗性水平。
展开▼
