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粗尾壁虎原尾细胞的建立与鉴定

Establishment and characterization of rough-tailed gecko original tail cells.

作者信息

Moghanjoghi Shiva Mohamadi, Ganjibakhsh Meysam, Gohari Neda Sadat, Izadpanah Mehrnaz, Rahmati Hedieh, Gorji Zahra Elyasi, Mohebali Nazanin, Vakhshiteh Faezeh, Farzaneh Parvaneh

机构信息

Human and Animal Cell Bank, Iranian Biological Resource Center (IBRC), ACECR, P. O. Box 1551916111, Tehran, Iran.

Department of Genetics, Faculty of Biological Sciences, Tarbiat Modares University, Tehran, Iran.

出版信息

Cytotechnology. 2018 Oct;70(5):1337-1347. doi: 10.1007/s10616-018-0223-7. Epub 2018 Jun 8.

Abstract

Some of lizard species have the ability to lose their tail in order to defend against predators and regenerate the new tail. Lizard's regenerated tail has attracted scientists' attention for unraveling the regeneration process, but less information is known about the cellular characterization and cell growth properties of original tail. This research aimed to report cell culture and banking process of rough-tailed gecko or Cyrtopodion scabrum's original tail cell sample from inner tissue without skin using tissue explant technique. For banking reports, it is essential to analyze this cells' potential to proliferate, to investigate biological aspects such as cell culture features, differentiation and chromosome number and to report its species identification and quality control. To achieve optimal growth conditions, three different temperatures for incubation including 18, 23 and 37 °C and two different media including DMEM and L-15 were applied. The expanded cells were studied for their potential to adipose and osteoblast differentiation. Results indicated that lizard's original tail cells could be successfully obtained by explant technique. The cells demonstrated fibroblast like morphology with population doubling times of approximately 24 ± 0.5 h. Karyotyping analysis showed a distribution of 2n = 40 chromosome number for this cell line. The comparison of different incubation media and temperatures showed that cell growth is equally optimal in all mentioned conditions according to growth curves. Adipose and osteoblast differentiation was obviously observed in these cells which confirms the hint of stem-ness in the produced mixed cells. According to cell banking policies, produced cells were also checked for bacterial, fungal, yeast and mycoplasma contaminations and no contamination was observed. Multiplex PCR for identification of species confirmed the species of lizard with no cross-contamination with other cells in the cell bank. Establishment of authenticated and well-characterized lizard's original tail cell line will provide a valuable source for subsequent in vitro regenerative research and molecular studies which are not feasible in in vivo methods. This finding will allow us to get an opportunity to create and preserve a new collection of lizard cell lines in the future.

摘要

一些蜥蜴物种能够通过断尾来抵御捕食者,并再生出新尾巴。蜥蜴的再生尾巴因有助于揭示再生过程而吸引了科学家的关注,但对于原尾巴的细胞特征和细胞生长特性却知之甚少。本研究旨在报告采用组织块培养技术,从无皮肤的粗尾沙虎(Cyrtopodion scabrum)原尾巴内部组织获取细胞样本并进行细胞库保存的过程。对于细胞库保存报告而言,分析这些细胞的增殖潜力、研究细胞培养特征、分化及染色体数目等生物学特性,并报告其物种鉴定和质量控制情况至关重要。为实现最佳生长条件,采用了三种不同的培养温度(18、23和37°C)以及两种不同的培养基(DMEM和L-15)。对扩增后的细胞进行了脂肪和成骨细胞分化潜力的研究。结果表明,通过组织块培养技术能够成功获取蜥蜴的原尾巴细胞。这些细胞呈现出成纤维细胞样形态,群体倍增时间约为24±0.5小时。核型分析显示该细胞系的染色体数目分布为2n = 40。不同培养温度和培养基的比较表明,根据生长曲线,在所有上述条件下细胞生长情况均最佳。在这些细胞中明显观察到了脂肪和成骨细胞分化,这证实了所产生的混合细胞具有干性特征。根据细胞库保存策略,还对所产生的细胞进行了细菌、真菌、酵母和支原体污染检测,未观察到污染情况。用于物种鉴定的多重PCR证实了蜥蜴的物种,且细胞库中未与其他细胞发生交叉污染。建立经过鉴定且特征明确的蜥蜴原尾巴细胞系将为后续体外再生研究和分子研究提供宝贵资源,而这些研究在体内方法中是不可行的。这一发现将使我们有机会在未来创建并保存一个新的蜥蜴细胞系库。

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