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Evolution of the osteoblast: skeletogenesis in gar and zebrafish

机译:成骨细胞的进化:和斑马鱼的骨骼生成

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Background Although the vertebrate skeleton arose in the sea 500 million years ago, our understanding of the molecular fingerprints of chondrocytes and osteoblasts may be biased because it is informed mainly by research on land animals. In fact, the molecular fingerprint of teleost osteoblasts differs in key ways from that of tetrapods, but we do not know the origin of these novel gene functions. They either arose as neofunctionalization events after the teleost genome duplication (TGD), or they represent preserved ancestral functions that pre-date the TGD. Here, we provide evolutionary perspective to the molecular fingerprints of skeletal cells and assess the role of genome duplication in generating novel gene functions. We compared the molecular fingerprints of skeletogenic cells in two ray-finned fish: zebrafish (Danio rerio)--a teleost--and the spotted gar (Lepisosteus oculatus)--a "living fossil" representative of a lineage that diverged from the teleost lineage prior to the TGD (i.e., the teleost sister group). We analyzed developing embryos for expression of the structural collagen genes col1a2, col2a1, col10a1, and col11a2 in well-formed cartilage and bone, and studied expression of skeletal regulators, including the transcription factor genes sox9 and runx2, during mesenchymal condensation. Results Results provided no evidence for the evolution of novel functions among gene duplicates in zebrafish compared to the gar outgroup, but our findings shed light on the evolution of the osteoblast. Zebrafish and gar chondrocytes both expressed col10a1 as they matured, but both species' osteoblasts also expressed col10a1, which tetrapod osteoblasts do not express. This novel finding, along with sox9 and col2a1 expression in developing osteoblasts of both zebrafish and gar, demonstrates that osteoblasts of both a teleost and a basally diverging ray-fin fish express components of the supposed chondrocyte molecular fingerprint. Conclusions Our surprising finding that the "chondrogenic" transcription factor sox9 is expressed in developing osteoblasts of both zebrafish and gar can help explain the expression of chondrocyte genes in osteoblasts of ray-finned fish. More broadly, our data suggest that the molecular fingerprint of the osteoblast, which largely is constrained among land animals, was not fixed during early vertebrate evolution.
机译:背景技术尽管脊椎动物骨架是在5亿年前出现在海洋中的,但我们对软骨细胞和成骨细胞分子指纹的理解可能会产生偏差,因为它主要是通过对陆地动物的研究获得的。实际上,硬骨成骨细胞的分子指纹与四足动物的分子指纹在关键方面有所不同,但我们不知道这些新型基因功能的起源。它们或者是在硬骨基因组复制(TGD)之后出现的新功能化事件,或者代表了TGD之前保留的祖先功能。在这里,我们提供了骨骼细胞分子指纹的进化观点,并评估了基因组复制在产生新型基因功能中的作用。我们比较了两种射线鳍鱼中的骨骼形成细胞的分子指纹:斑马鱼(Danio rerio)(一种硬骨鱼)和斑点(活的化石),代表了一种不同于硬骨鱼的世系。 TGD之前的血统(即硬骨姐妹组)。我们分析发育中的胚胎在结构良好的软骨和骨骼中表达结构性胶原基因col1a2,col2a1,col10a1和col11a2,并研究了间充质凝结过程中骨骼调节因子的表达,包括转录因子基因sox9和runx2。结果结果没有提供证据表明与gar外群相比,斑马鱼基因重复中新功能的进化,但是我们的发现为成骨细胞的进化提供了启示。斑马鱼和软骨细胞成熟时都表达col10a1,但是两个物种的成骨细胞也表达col10a1,而四足动物成骨细胞不表达。这一新发现以及在斑马鱼和gar发育中的成骨细胞中的sox9和col2a1表达,表明硬骨鱼和基底发散的鳍鳍鱼的成骨细胞都表达了所谓的软骨细胞分子指纹的成分。结论我们令人惊讶的发现表明,“成软骨”转录因子sox9在斑马鱼和gar的发育成骨细胞中表达,这可以解释软骨鱼成骨细胞中软骨细胞基因的表达。更广泛地说,我们的数据表明,成骨细胞的分子指纹主要在陆地动物中受到限制,在脊椎动物早期进化过程中并未固定。

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