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肺孢子菌表达一种活性的 Rtt109 组蛋白乙酰转移酶。

Pneumocystis carinii expresses an active Rtt109 histone acetyltransferase.

机构信息

Thoracic Diseases Research Unit, Department of Medicine and Department of Biochemistry, Mayo Clinic, Rochester, MN 55905, USA.

出版信息

Am J Respir Cell Mol Biol. 2011 Jun;44(6):768-76. doi: 10.1165/rcmb.2009-0443OC. Epub 2010 Jul 23.

Abstract

Species in the genus Pneumocystis can cause severe pneumonia in immune-compromised hosts. The identification of specific targets present in Pneumocystis species, but lacking in mammalian hosts, is paramount to developing new means to treat this infection. One such potential protein is Rtt109, which is a type of histone acetyltransferase (HAT) required for DNA replication in fungi, but not found in mammals. Sequence orthologues of Rtt109 are present in other fungi, but are absent in mammals, making it a potential pan-specific target against medically relevant fungi. Accordingly, we sought to identify the presence of an Rtt109 in P. carinii. A Pneumocystis carinii (Pc) Rtt109 165-bp partial sequence was initially identified from the incomplete P. carinii genome database. Subsequently, a full-length, 1,128-bp cDNA with homology to Saccharomyces cerevisiae Rtt109 (39% Basic Local Alignment Search Tool (BLASTP)) was cloned and characterized. Sequence analysis of PcRtt109 indicated that the P. carinii molecule contains the putative catalytic aspartate present in yeast. We further demonstrated that the PcRtt109 expressed in rtt109Δ S. cerevisiae cells restored H3-K56 acetylation and the sensitivity toward DNA-damaging agents of rtt109Δ mutant cells. Purified PcRtt109 had the ability to acetylate lysine-56 of histone H3, similar to the ability of Schizosaccharomyces pombe Rtt109 protein. The site-directed mutagenesis of PcRtt109 D84A, a potential regulatory site in the Rtt109 HAT family, abolished H3 acetylation, whereas a DD218/219AA mutation that compromised the activity of ScRtt109 had little effect, demonstrating similarities and differences in Pneumocystis PcRtt109 compared with yeast Saccharomyces cerevisiae Rtt109. These results indicate that P. carinii contains an Rtt109 HAT molecule, and represent the complete identification and characterization of a HAT molecule from this important opportunistic fungal pathogen.

摘要

肺囊虫属的物种可导致免疫功能低下宿主发生严重肺炎。鉴定肺囊虫属物种中存在的特定靶标,但在哺乳动物宿主中不存在,这对于开发治疗这种感染的新方法至关重要。Rtt109 就是这样一种潜在的蛋白质,它是一种组蛋白乙酰转移酶 (HAT),是真菌中 DNA 复制所必需的,但在哺乳动物中不存在。Rtt109 的序列同源物存在于其他真菌中,但在哺乳动物中不存在,使其成为针对医学相关真菌的潜在泛特异性靶标。因此,我们试图确定肺囊虫属中是否存在 Rtt109。最初从不完全的肺囊虫属基因组数据库中鉴定出肺囊虫属 (Pc) Rtt109 的 165 个碱基对的部分序列。随后,克隆并表征了全长 1128 个碱基对的 cDNA,与酿酒酵母 Rtt109 具有同源性 (39%基本局部比对搜索工具 (BLASTP))。PcRtt109 的序列分析表明,肺囊虫属分子包含酵母中存在的假定催化天冬氨酸。我们进一步证明,在 rtt109Δ酿酒酵母细胞中表达的 PcRtt109 恢复了 H3-K56 乙酰化,并恢复了 rtt109Δ 突变细胞对 DNA 损伤剂的敏感性。纯化的 PcRtt109 具有乙酰化组蛋白 H3 赖氨酸-56 的能力,类似于裂殖酵母 Rtt109 蛋白的能力。PcRtt109 D84A 的定点突变,Rtt109 HAT 家族中的一个潜在调节位点,消除了 H3 乙酰化,而 ScRtt109 的活性受到影响的 DD218/219AA 突变几乎没有影响,这表明与酵母酿酒酵母 Rtt109 相比,肺囊虫属 PcRtt109 存在相似之处和差异。这些结果表明,肺囊虫属含有一种 Rtt109 HAT 分子,代表了这种重要的机会性真菌病原体中 HAT 分子的完整鉴定和表征。

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