Structural analysis of a bacterial UDP-sugar 2-epimerase reveals the active site architecture before and after catalysis.

The Journal of Biological Chemistry Pub Date : 2023-10-01 Epub Date: 2023-09-03 DOI:10.1016/j.jbc.2023.105200
James B Thoden, James O McKnight, Charles W Kroft, Joshua D T Jast, Hazel M Holden
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Abstract

The sugar, 2,3-diacetamido-2,3-dideoxy-d-mannuronic acid, was first identified ∼40 years ago in the O-antigen of Pseudomonas aeruginosa O:3,a,d. Since then, it has been observed on the O-antigens of various pathogenic Gram-negative bacteria including Bordetella pertussis, Escherichia albertii, and Pseudomonas mediterranea. Previous studies have established that five enzymes are required for its biosynthesis beginning with uridine dinucleotide (UDP)-N-acetyl-d-glucosamine (UDP-GlcNAc). The final step in the pathway is catalyzed by a 2-epimerase, which utilizes UDP-2,3-diacetamido-2,3-dideoxy-d-glucuronic acid as its substrate. Curious as to whether this biochemical pathway is found in extreme thermophiles, we examined the published genome sequence for Thermus thermophilus HB27 and identified five ORFs that could possibly encode for the required enzymes. The focus of this investigation is on the ORF WP_011172736, which we demonstrate encodes for a 2-epimerase. For this investigation, ten high resolution X-ray crystallographic structures were determined to resolutions of 2.3 Å or higher. The models have revealed the manner in which the 2-epimerase anchors its UDP-sugar substrate as well as its UDP-sugar product into the active site. In addition, this study reveals for the first time the manner in which any sugar 2-epimerase can simultaneously bind UDP-sugars in both the active site and the allosteric binding region. We have also demonstrated that the T. thermophilus enzyme is allosterically regulated by UDP-GlcNAc. Whereas the sugar 2-epimerases that function on UDP-GlcNAc have been the focus of past biochemical and structural analyses, this is the first detailed investigation of a 2-epimerase that specifically utilizes UDP-2,3-diacetamido-2,3-dideoxy-d-glucuronic acid as its substrate.

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细菌UDP糖2-二聚酶的结构分析揭示了催化前后的活性位点结构。
这种糖,2,3-二乙酰氨基-2,3-二脱氧-d-甘露糖醛酸,大约40年前首次在铜绿假单胞菌O:3,a,d的O抗原中被鉴定。从那时起,它已经在各种致病性革兰氏阴性菌的O抗原上被观察到,包括百日咳杆菌、艾伯氏大肠杆菌和地中海假单胞菌。先前的研究已经确定,从尿苷二核苷酸(UDP)-N-乙酰-d-葡糖胺(UDP-GlcNAc)开始,其生物合成需要五种酶。该途径的最后一步由2-庚二酸酶催化,该酶利用UDP-2,3-二乙酰氨基-2,3-二脱氧-d-葡萄糖醛酸作为底物。出于对这种生物化学途径是否在极端嗜热菌中发现的好奇,我们检查了已发表的嗜热菌HB27的基因组序列,并鉴定了五个可能编码所需酶的ORF。本研究的重点是ORF WP_011172736,我们证明它编码2-单聚酶。在这项研究中,10个高分辨率X射线晶体结构被确定为2.3Å或更高的分辨率。该模型揭示了2-二甲基酶将其UDP糖底物及其UDP糖产物锚定到活性位点的方式。此外,这项研究首次揭示了任何糖2-二聚酶可以同时在活性位点和变构结合区结合UDP糖的方式。我们还证明嗜热T.thermophilus酶是由UDP-GlcNAc变构调节的。尽管对UDP-GlcNAc起作用的糖2-二聚体酶一直是过去生化和结构分析的焦点,但这是首次对专门利用UDP-2,3-二乙酰氨基-2,3-二脱氧-d-葡萄糖醛酸作为底物的2-二聚物酶进行详细研究。
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