Fanomezana M. Ranaivoson , Rieke Bande , Isabell Cardaun , Antonio De Riso , Annette Gärtner , Pui Loke , Christina Reinisch , Prasuna Vogirala , Edward Beaumont , J. L. Smith (Editor)
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It belongs to the peptidylarginine deiminase (PAD) enzyme family that catalyzes the conversion of arginine residues to citrulline in proteins. In contrast to other members of the family, recombinant PAD6 was previously found to be catalytically inactive. We sought to provide structural insight into the human homologue to shed light on this observation. We report here the first crystal structure of PAD6, determined at 1.7 Å resolution. PAD6 follows the same domain organization as other structurally known PAD isoenzymes. Further structural analysis and size-exclusion chromatography show that PAD6 behaves as a homodimer similar to PAD4. Differential scanning fluorimetry suggests that PAD6 does not coordinate Ca<sup>2+</sup> which agrees with acidic residues found to coordinate Ca<sup>2+</sup> in other PAD homologs not being conserved in PAD6. The crystal structure of PAD6 shows similarities with the inactive state of <em>apo</em> PAD2, in which the active site conformation is unsuitable for catalytic citrullination. The putative active site of PAD6 adopts a non-productive conformation that would not allow protein–substrate binding due to steric hindrance with rigid secondary structure elements. This observation is further supported by the lack of activity on the histone H3 and cytokeratin 5 substrates. 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The putative active site of PAD6 adopts a non-productive conformation that would not allow protein–substrate binding due to steric hindrance with rigid secondary structure elements. This observation is further supported by the lack of activity on the histone H3 and cytokeratin 5 substrates. 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引用次数: 0
摘要
人类肽基精氨酸脱氨酶同工酶 VI(PAD6)主要局限于哺乳动物卵巢组织中卵母细胞的细胞质晶格中,对女性生育至关重要。它属于肽基精氨酸脱氨酶(PAD)酶家族,能催化蛋白质中的精氨酸残基转化为瓜氨酸。与该家族的其他成员不同,重组 PAD6 先前被发现没有催化活性。我们试图通过人类同源物的结构来揭示这一现象。我们在此报告了以 1.7 Å 分辨率测定的 PAD6 的首个晶体结构。PAD6 与其他结构上已知的 PAD 同工酶具有相同的结构域组织。进一步的结构分析和尺寸排阻色谱法显示,PAD6 表现为与 PAD4 相似的同源二聚体。差示扫描荧光测定法表明,PAD6 并不协调 Ca2+,这与在其他 PAD 同源物中发现的协调 Ca2+的酸性残基在 PAD6 中没有保留一致。PAD6 的晶体结构显示与 apo PAD2 的非活性状态相似,其中活性位点构象不适合催化瓜氨酸化。PAD6 的推定活性位点采用了非生产性构象,由于与刚性二级结构元素之间的立体阻碍,无法实现蛋白质与底物的结合。组蛋白 H3 和细胞角蛋白 5 底物缺乏活性进一步证实了这一观点。这些发现表明,与其他 PADs 相比,PAD6 的酶激活机制不同;或者,PAD6 可能在卵母细胞和早期胚胎的细胞质晶格中发挥非酶功能。
Crystal structure of human peptidylarginine deiminase type VI (PAD6) provides insights into its inactivity
The human peptidylarginine deiminase type VI (PAD6) is essential in oocyte and embryonic development as a component of the supramolecular assemblies called cytoplasmic lattices. The crystal structure presented here suggests PAD6 assembles as a dimer resembling other PADs, albeit with compromised abilities to bind Ca2+ and substrates. This aligns with existing in vitro data which indicate an enzymatically inactive isoform of PAD.
Human peptidylarginine deiminase isoform VI (PAD6), which is predominantly limited to cytoplasmic lattices in the mammalian oocytes in ovarian tissue, is essential for female fertility. It belongs to the peptidylarginine deiminase (PAD) enzyme family that catalyzes the conversion of arginine residues to citrulline in proteins. In contrast to other members of the family, recombinant PAD6 was previously found to be catalytically inactive. We sought to provide structural insight into the human homologue to shed light on this observation. We report here the first crystal structure of PAD6, determined at 1.7 Å resolution. PAD6 follows the same domain organization as other structurally known PAD isoenzymes. Further structural analysis and size-exclusion chromatography show that PAD6 behaves as a homodimer similar to PAD4. Differential scanning fluorimetry suggests that PAD6 does not coordinate Ca2+ which agrees with acidic residues found to coordinate Ca2+ in other PAD homologs not being conserved in PAD6. The crystal structure of PAD6 shows similarities with the inactive state of apo PAD2, in which the active site conformation is unsuitable for catalytic citrullination. The putative active site of PAD6 adopts a non-productive conformation that would not allow protein–substrate binding due to steric hindrance with rigid secondary structure elements. This observation is further supported by the lack of activity on the histone H3 and cytokeratin 5 substrates. These findings suggest a different mechanism for enzymatic activation compared with other PADs; alternatively, PAD6 may exert a non-enzymatic function in the cytoplasmic lattice of oocytes and early embryos.
期刊介绍:
IUCrJ is a new fully open-access peer-reviewed journal from the International Union of Crystallography (IUCr).
The journal will publish high-profile articles on all aspects of the sciences and technologies supported by the IUCr via its commissions, including emerging fields where structural results underpin the science reported in the article. Our aim is to make IUCrJ the natural home for high-quality structural science results. Chemists, biologists, physicists and material scientists will be actively encouraged to report their structural studies in IUCrJ.
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