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后生动物基于 Ca++的骨架的常见遗传因素:破骨细胞刺激因子和碳酸酐酶在钙质海绵中的作用。

Common genetic denominators for Ca++-based skeleton in Metazoa: role of osteoclast-stimulating factor and of carbonic anhydrase in a calcareous sponge.

机构信息

ERC Advanced Investigator Grant Research Group at Institute for Physiological Chemistry, University Medical Center of the Johannes Gutenberg University Mainz, Mainz, Germany.

出版信息

PLoS One. 2012;7(4):e34617. doi: 10.1371/journal.pone.0034617. Epub 2012 Apr 10.

Abstract

Calcium-based matrices serve predominantly as inorganic, hard skeletal systems in Metazoa from calcareous sponges [phylum Porifera; class Calcarea] to proto- and deuterostomian multicellular animals. The calcareous sponges form their skeletal elements, the spicules, from amorphous calcium carbonate (ACC). Treatment of spicules from Sycon raphanus with sodium hypochlorite (NaOCl) results in the disintegration of the ACC in those skeletal elements. Until now a distinct protein/enzyme involved in ACC metabolism could not been identified in those animals. We applied the technique of phage display combinatorial libraries to identify oligopeptides that bind to NaOCl-treated spicules: those oligopeptides allowed us to detect proteins that bind to those spicules. Two molecules have been identified, the (putative) enzyme carbonic anhydrase and the (putative) osteoclast-stimulating factor (OSTF), that are involved in the catabolism of ACC. The complete cDNAs were isolated and the recombinant proteins were prepared to raise antibodies. In turn, immunofluorescence staining of tissue slices and qPCR analyses have been performed. The data show that sponges, cultivated under standard condition (10 mM CaCl(2)) show low levels of transcripts/proteins for carbonic anhydrase or OSTF, compared to those animals that had been cultivated under Ca(2+)-depletion condition (1 mM CaCl(2)). Our data identify with the carbonic anhydrase and the OSTF the first two molecules which remain conserved in cells, potentially involved in Ca-based skeletal dissolution, from sponges (sclerocytes) to human (osteoclast).

摘要

钙基基质主要作为无机组分存在于后生动物的硬骨骼系统中,从钙质海绵动物门(多孔动物门;钙质纲)到原口动物和后口动物多细胞动物。钙质海绵动物用无定形碳酸钙(ACC)形成它们的骨骼元素,骨针。用次氯酸钠(NaOCl)处理 Sycon raphanus 的骨针会导致这些骨骼元素中的 ACC 解体。到目前为止,还没有在这些动物中鉴定出与 ACC 代谢有关的特定蛋白质/酶。我们应用噬菌体展示组合文库技术来鉴定与 NaOCl 处理的骨针结合的寡肽:这些寡肽使我们能够检测到与这些骨针结合的蛋白质。已经鉴定出两种分子,即(假定)碳酸酐酶和(假定)破骨细胞刺激因子(OSTF),它们参与 ACC 的分解代谢。分离出了完整的 cDNA,并制备了重组蛋白以产生抗体。反过来,对组织切片进行免疫荧光染色和 qPCR 分析。数据表明,与在标准条件(10 mM CaCl2)下培养的海绵相比,在 Ca2+耗尽条件(1 mM CaCl2)下培养的海绵中碳酸酐酶或 OSTF 的转录本/蛋白水平较低。我们的数据确定了碳酸酐酶和 OSTF 这两种分子,它们是第一个在细胞中保守的、潜在参与基于 Ca 的骨骼溶解的分子,从海绵(骨细胞)到人类(破骨细胞)都是如此。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8249/3323548/b5e18b9360af/pone.0034617.g001.jpg

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