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首页> 外文期刊>Journal of bacteriology >Transcriptional Regulation of the Gene Cluster Encoding Allantoinase and Guanine Deaminase in Klebsiella pneumoniae
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Transcriptional Regulation of the Gene Cluster Encoding Allantoinase and Guanine Deaminase in Klebsiella pneumoniae

机译:肺炎克雷伯菌中尿囊素酶和鸟嘌呤脱氨酶基因簇的转录调控。

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Purines can be used as the sole source of nitrogen by several strains of K. pneumoniae under aerobic conditions. The genes responsible for the assimilation of purine nitrogens are distributed in three separated clusters in the K. pneumoniae genome. Here, we characterize the cluster encompassing genes KPN_01787 to KPN_01791, which is involved in the conversion of allantoin into allantoate and in the deamination of guanine to xanthine. These genes are organized in three transcriptional units, hpxSAB, hpxC, and guaD. Gene hpxS encodes a regulatory protein of the GntR family that mediates regulation of this system by growth on allantoin. Proteins encoded by hpxB and guaD display allantoinase and guanine deaminase activity, respectively. In this cluster, hpxSAB is the most tightly regulated unit. This operon was activated by growth on allantoin as a nitrogen source; however, addition of allantoin to nitrogen excess cultures did not result in hpxSAB induction. Neither guaD nor hpxC was induced by allantoin. Expression of guaD is mainly regulated by nitrogen availability through the action of NtrC. Full induction of hpxSAB by allantoin requires both HpxS and NAC. HpxS may have a dual role, acting as a repressor in the absence of allantoin and as an activator in its presence. HpxS binds to tandem sites, S1 and S2, overlapping the ?10 and ?35 sequences of the hpxSAB promoter, respectively. The NAC binding site is located between S1 and S2 and partially overlaps S2. In the presence of allantoin, interplay between NAC and HpxS is proposed.
机译:嘌呤可以在好氧条件下被几种肺炎克雷伯菌用作唯一的氮源。负责嘌呤氮同化的基因分布在肺炎克雷伯菌基因组的三个单独的簇中。在这里,我们表征包含基因KPN_01787至KPN_01791的簇,该簇涉及尿囊素向尿囊酸的转化以及鸟嘌呤向黄嘌呤的脱氨基。这些基因分为三个转录单位,分别是 hpxSAB hpxC guaD 。基因 hpxS 编码GntR家族的调节蛋白,该蛋白通过尿囊素的生长介导对该系统的调节。由 hpxB guaD 编码的蛋白质分别显示尿囊素酶和鸟嘌呤脱氨酶活性。在此群集中, hpxSAB 是监管最严格的单元。该操纵子通过尿囊素作为氮源的生长而被激活。但是,将尿囊素添加到氮过量的培养物中不会导致 hpxSAB 的诱导。尿囊素既没有诱导 guaD 也没有诱导 hpxC 。 guaD 的表达主要受NtrC作用下氮素有效性的调控。尿囊素完全诱导 hpxSAB 既需要HpxS也需要NAC。 HpxS可能具有双重作用,在没有尿囊素的情况下起阻遏剂的作用,在存在尿囊素的情况下起激活剂的作用。 HpxS绑定到串联位点S1和S2,分别与 hpxSAB 启动子的10和35序列重叠。 NAC结合位点位于S1和S2之间,与S2部分重叠。在尿囊素的存在下,提出了NAC和HpxS之间的相互作用。

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