Mycobacterium tuberculosis Mce3R TetR-like Repressor Forms an Asymmetric Four-Helix Bundle and Binds a Nonpalindrome Sequence†.

IF 3.5 2区生物学 Q2 BIOCHEMISTRY & MOLECULAR BIOLOGY

ACS Chemical Biology Pub Date : 2024-11-15 DOI:10.1021/acschembio.4c00687

Navanjalee T Panagoda, Gábor Balázsi, Nicole S Sampson

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引用次数: 0

Abstract

Mycobacterium tuberculosis (Mtb), the causative agent of tuberculosis, is a major global health concern. TetR family repressors (TFRs) are important for Mtb's adaptation to the human host environment. Our study focuses on one notable Mtb repressor, Mce3R, composed of an unusual double TFR motif. Mce3R-regulated genes encode enzymes implicated in cholesterol metabolism, resistance against reactive oxygen species, and lipid transport activities important for Mtb survival and persistence in the host and for the cellular activity of a 6-azasteroid derivative. Here, we present the structure of Mce3R bound to its DNA operator, unveiling a unique asymmetric assembly previously unreported. We obtained a candidate DNA-binding motif through MEME motif analysis, comparing intergenic regions of mce3R orthologues and identifying nonpalindromic regions conserved between orthologues. Using an electrophoretic mobility shift assay (EMSA), we confirmed that Mce3R binds to a 123-bp sequence that includes the predicted motif. Using scrambled DNA and DNA oligonucleotides of varying lengths with sequences from the upstream region of the yrbE3A (mce3) operon, we elucidated the operator region to be composed of two Mce3R binding sites, each a 25-bp asymmetric sequence separated by 53 bp. Mce3R binds with a higher affinity to the downstream site with a K_d of 2.4 ± 0.7 nM. The cryo-EM structure of Mce3R bound to the 123-bp sequence was refined to a resolution of 2.51 Å. Each Mce3R monomer comprises 21 α-helices (α1-α21) folded into an asymmetric TFR-like structure with a core asymmetric four-helix bundle. This complex has two nonidentical HTH motifs and a single ligand-binding domain. The two nonidentical HTHs from each TFR bind within the high-affinity, nonpalindromic operator motif, with Arg53 and Lys262 inserted into the major groove. Site-directed mutagenesis of Arg53 to alanine abrogated DNA binding, validating the Mce3R/DNA structure obtained. Among 811,645 particles, 63% were Mce3R homodimer bound to two duplex oligonucleotides. Mce3R homodimerizes primarily through α15, and each monomer binds to an identical site in the DNA duplex oligonucleotide.

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结核分枝杆菌 Mce3R TetR 样抑制因子形成不对称的四螺旋体束并结合非标词序列†。

结核分枝杆菌（Mtb）是结核病的病原体，是全球关注的主要健康问题。TetR家族抑制因子（TFR）对于Mtb适应人类宿主环境非常重要。我们的研究重点是一种著名的 Mtb 抑制因子 Mce3R，它由一个不寻常的双 TFR 基序组成。Mce3R调控的基因编码与胆固醇代谢、抗活性氧和脂质转运活动有关的酶，这些活动对Mtb在宿主体内的生存和持久性以及6-氮杂甾类衍生物的细胞活性非常重要。在这里，我们展示了 Mce3R 与其 DNA 操作体结合的结构，揭示了一种以前从未报道过的独特的不对称组装。我们通过 MEME 动点分析获得了一个候选 DNA 结合动点，比较了 mce3R 同源物的基因间区域，并确定了同源物之间的非首尾对称区域。通过电泳迁移试验（EMSA），我们证实了 Mce3R 与一个 123 bp 的序列结合，该序列包括预测的基调。利用来自yrbE3A（mce3）操作子上游区域序列的乱序 DNA 和不同长度的 DNA 寡核苷酸，我们阐明了操作子区域由两个 Mce3R 结合位点组成，每个位点都是 25 bp 的不对称序列，中间相隔 53 bp。Mce3R 与下游位点的结合亲和力较高，Kd 为 2.4 ± 0.7 nM。每个 Mce3R 单体由 21 个 α-螺旋（α1-α21）组成，折叠成不对称的 TFR 样结构，其核心是不对称的四螺旋束。该复合物有两个非相同的 HTH 主题和一个配体结合域。每个 TFR 的两个非相同 HTH 在高亲和性、非全向的操作者图案内结合，Arg53 和 Lys262 插入主沟。将 Arg53 定点突变为丙氨酸可抑制 DNA 结合，从而验证了所获得的 Mce3R/DNA 结构。在811,645个颗粒中，63%是与两个双链寡核苷酸结合的Mce3R同源二聚体。Mce3R 主要通过 α15 进行同源二聚体化，每个单体都与 DNA 双链寡核苷酸中的一个相同位点结合。

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来源期刊

ACS Chemical Biology 生物-生化与分子生物学

CiteScore

7.50

自引率

5.00%

发文量

353

审稿时长

3.3 months

期刊介绍： ACS Chemical Biology provides an international forum for the rapid communication of research that broadly embraces the interface between chemistry and biology. The journal also serves as a forum to facilitate the communication between biologists and chemists that will translate into new research opportunities and discoveries. Results will be published in which molecular reasoning has been used to probe questions through in vitro investigations, cell biological methods, or organismic studies. We welcome mechanistic studies on proteins, nucleic acids, sugars, lipids, and nonbiological polymers. The journal serves a large scientific community, exploring cellular function from both chemical and biological perspectives. It is understood that submitted work is based upon original results and has not been published previously.