Cellulose binding and the timing of expression influence protein targeting to the double-layered cyst wall of Acanthamoeba.

IF 3.7 2区 生物学 Q2 MICROBIOLOGY mSphere Pub Date : 2024-09-25 Epub Date: 2024-08-13 DOI:10.1128/msphere.00466-24
Bharath Kanakapura Sundararaj, Manish Goyal, John Samuelson
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Abstract

The cyst wall of the eye pathogen Acanthamoeba castellanii contains cellulose and has ectocyst and endocyst layers connected by conical ostioles. Cyst walls contain families of lectins that localize to the ectocyst layer (Jonah) or the endocyst layer and ostioles (Luke and Leo). How lectins and an abundant laccase bind cellulose and why proteins go to locations in the wall are not known and are the focus of the studies here. Structural predictions identified β-jelly-roll folds (BJRFs) of Luke and sets of four disulfide knots (4DKs) of Leo, each of which contains linear arrays of aromatic amino acids, also present in carbohydrate-binding modules of bacterial and plant endocellulases. Ala mutations showed that these aromatics are necessary for cellulose binding and proper localization of Luke and Leo in the Acanthamoeba cyst wall. BJRFs of Luke, 4DKs of Leo, a single β-helical fold (BHF) of Jonah, and a copper oxidase domain of the laccase each bind to glycopolymers in both layers of deproteinated cyst walls. Promoter swaps showed that ectocyst localization does not just correlate with but is caused by early encystation-specific expression, while localization in the endocyst layer and ostioles is caused by later expression. Evolutionary studies showed distinct modes of assembly of duplicated domains in Luke, Leo, and Jonah lectins and suggested Jonah BHFs originated from bacteria, Luke BJRFs share common ancestry with slime molds, while 4DKs of Leo are unique to Acanthamoeba.IMPORTANCEAcanthamoebae is the only human parasite with cellulose in its cyst wall and conical ostioles that connect its inner and outer layers. Cyst walls are important virulence factors because they make Acanthamoebae resistant to surface disinfectants, hand sanitizers, contact lens sterilizers, and antibiotics applied to the eye. The goal here was to understand better how proteins are targeted to specific locations in the cyst wall. To this end, we identified three new proteins in the outer layer of the cyst wall, which may be targets for diagnostic antibodies in corneal scrapings. We used structural predictions and mutated proteins to show linear arrays of aromatic amino acids of two unrelated wall proteins are necessary for binding cellulose and proper wall localization. We showed early expression during encystation causes proteins to localize to the outer layer, while later expression causes proteins to localize to the inner layer and the ostioles.

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纤维素结合和表达时间影响蛋白在棘阿米巴双层囊壁的靶向性。
眼部病原体棘阿米巴(Acanthamoeba castellanii)的囊壁含有纤维素,外囊层和内囊层由圆锥形骨管连接。囊壁含有凝集素家族,这些凝集素定位于外囊层(约拿)或内囊层和囊管层(卢克和利奥)。凝集素和一种丰富的漆酶如何与纤维素结合,以及为什么蛋白质会定位于囊壁的各个位置,这些都是未知的,也是本文研究的重点。结构预测发现了 Luke 的β-果冻状褶皱(BJRFs)和 Leo 的四组二硫结(4DKs),每组二硫结都包含芳香族氨基酸的线性阵列,这些芳香族氨基酸也存在于细菌和植物内纤维素酶的碳水化合物结合模块中。Ala突变表明,这些芳香族氨基酸是纤维素结合以及Luke和Leo在棘阿米巴囊壁中正确定位所必需的。Luke的BJRFs、Leo的4DKs、Jonah的单个β-螺旋折叠(BHF)以及漆酶的铜氧化酶结构域分别与脱蛋白囊壁两层中的糖聚合物结合。启动子交换表明,外囊定位不仅与囊壁特异性表达有关,而且是由早期囊壁特异性表达引起的,而内囊层和骨管的定位则是由后期表达引起的。进化研究显示,Luke、Leo 和 Jonah 凝集素中重复结构域的组装模式各不相同,并表明 Jonah BHFs 起源于细菌,Luke BJRFs 与粘菌有着共同的祖先,而 Leo 的 4DKs 则是棘阿米巴所独有的。囊壁是重要的致病因子,因为它们使棘阿米巴原虫对表面消毒剂、手部消毒剂、隐形眼镜消毒剂和眼部使用的抗生素具有抵抗力。我们的目标是更好地了解蛋白质如何靶向囊壁的特定位置。为此,我们在囊壁外层发现了三种新蛋白质,它们可能是角膜刮片中诊断抗体的靶标。我们利用结构预测和突变蛋白表明,两种不相关的囊壁蛋白的芳香族氨基酸线性阵列是结合纤维素和正确定位囊壁所必需的。我们发现,在角膜囊变过程中,早期表达会导致蛋白质定位到外层,而后期表达则会导致蛋白质定位到内层和骨膜。
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来源期刊
mSphere
mSphere Immunology and Microbiology-Microbiology
CiteScore
8.50
自引率
2.10%
发文量
192
审稿时长
11 weeks
期刊介绍: mSphere™ is a multi-disciplinary open-access journal that will focus on rapid publication of fundamental contributions to our understanding of microbiology. Its scope will reflect the immense range of fields within the microbial sciences, creating new opportunities for researchers to share findings that are transforming our understanding of human health and disease, ecosystems, neuroscience, agriculture, energy production, climate change, evolution, biogeochemical cycling, and food and drug production. Submissions will be encouraged of all high-quality work that makes fundamental contributions to our understanding of microbiology. mSphere™ will provide streamlined decisions, while carrying on ASM''s tradition for rigorous peer review.
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