两种细胞来源的21-三体综合征诱导多能干细胞系的建立及比较

21-三体综合征是染色体异常导致的疾病,通过重编程21-三体综合征患儿两种组织来源的细胞成为多能干细胞,比较两种组织来源的细胞建立21-三体综合征诱导多能干细胞（T21-iPSCs）系的效率,为进一步研究21-三体综合征发病机制提供细胞模型,并为选择高效制备T21-iPSCs的组织类型提供理论依据。该实验利用慢病毒介导4种转录因子（Oct4、Sox2、Klf4、c-Myc）分别诱导人21-三体综合征的羊水细胞和胎儿皮肤成纤维细胞,建立诱导多能干细胞系（Trisomy 21 human amniotic fl uid induced pluripotent stem cells,T21 hAF-iPSCs;Trisomy 21 human dermal fi broblast induced pluripotent stem cells,T21 hDF-iPSCs）,T21 hAF-iPSCs及T21 hDF-iPSCs在蛋白和mRNA水平上均表达人胚胎干细胞的多能性分子标记,如Oct4、Nanog等,具有在体外及体内分化三个胚层的能力,其在培养过程中能维持异常核型并能维持自我更新状态。结果发现,利用羊水细胞建立T21-iPSCs效率高于皮肤成纤维细胞,羊水细胞可能是制备T21-iPSCs的理想细胞类型。     

建立人类异常染色体核型的成纤维细胞系及滋养层细胞系

从自然流产绒毛或者中期妊娠羊水中分离细胞体外培养, 建立人类异常染色体核型成纤维细胞系及滋养层细胞系.中期妊娠羊水染色体诊断或自然流产绒毛染色体诊断过程中, 行G显带细胞核型分型, 对于发现异常核型的细胞, 进行分离、培养、传代、冻存、复苏及鉴定, 建立细胞系, 用PowerPlex 16系统行DNA-STR基因型检测.建立1株来自羊水的21三体成纤维细胞系, 以及7株来自绒毛的滋养层细胞系, 核型分别为47, XX 21; 69, XXX; 69, XXY; 47, XY 12; 47, XX 5; 48, XY 21, 22; 47, XY 18.所有细胞系体外传代均超过10代, 冷冻复苏率大于50%, 核型维持稳定, DNA-STR基因检测能对人细胞系进行个体识别.人异常染色体核型的成纤维细胞系和绒毛膜滋养层细胞系的建立,可以为探讨异常染色体产生机制及相关的分子遗传学研究提供细胞来源.     

人诱导性多潜能干细胞(iPS细胞)系的建立

掌握建立人iPS细胞系(induced pluripotent stem cells,iPSCs)的技术,以便为人肿瘤细胞重编程为iPS细胞建立技术平台.在人胚胎干细胞的培养条件下,通过携带Oct4、Sox2、c-Myc、Klf44个混合因子的慢病毒感染人皮肤成纤维细胞(CCD-1079SK细胞),从而诱导成干细胞样的克隆.根据人胚胎干细胞的特性进行如下鉴定:克隆形态、碱性磷酸酶活性、核型和CCD-1079SK细胞来源的克隆拟胚体(embryoid bodies,EBs)形成及分化等.结果显示,在人胚胎干细胞的培养环境中,导入Oct4、Sox2、c-Myc、Klf44个因子的CCD-1079SK细胞产生了一株iPSC克隆,这株iPSC克隆在细胞形态、增殖能力、胚胎细胞特异性表面抗原以及基因表达与人胚胎干细胞相似,此外,iPSC克隆在体外悬浮培养中形成拟胚体并分化成3个胚层.人iPS细胞系的成功建立为利用iPS细胞技术开展肿瘤细胞重编程研究奠定了坚实基础.     

一种获得猪诱导性多能干细胞的新方法

诱导性多能干细胞技术表明,通过过表达4个重编程因子可使体细胞逆转到多能性的状态,为建立更多家畜动物的多能性干细胞系提供了新的方法,如猪、牛、羊等农业动物.莫洛尼氏鼠白血病逆转录病毒载体被广泛应用于小鼠iPS细胞的建系和机制研究上,然而这种病毒只能感染小鼠和大鼠细胞,这限制了它在其他哺乳动物iPS细胞系建立上的应用.本实验采用一种新的逆转录病毒系统,可以高效便捷地从猪成纤维细胞中获得iPS细胞.通过在GP2-293细胞中包装VSV-G蛋白包被的病毒,仅一步感染猪成纤维细胞即可转入4个人源重编程因子（Oct4,Sox2,Klf4和c-Myc）.在添加有碱性成骨因子bFGF的人类胚胎干细胞培养体系中,成功建立6株和人类胚胎干细胞形态极其相似的猪iPS细胞系.这些猪iPS克隆具有较大的细胞核/细胞质比例、边界清晰、细胞呈扁平状等特征.在体外可以分化成拟胚体,注射入免疫缺陷性小鼠体内可以形成畸胎瘤,含有3种胚层类型的组织.     

无饲养层和动物源蛋白的β-地中海贫血诱导多能干细胞系的建立

β-地中海贫血患者因无合适的造血干细胞供体来源从而不得不靠输血维持生命。诱导多能干细胞(iPS)技术为获得患者自身遗传背景的干细胞进行临床治疗开拓了新途径。目前,建立iPS细胞系的过程需要使用小鼠胚胎成纤维细胞作为饲养层和动物源的蛋白成分,因此建立的iPS细胞系存在病原体和动物源蛋白污染的可能性,不能应用于临床。采用目前商品化的TeSRTM2和StemAdhereTMDefined Matrix限定培养体系,利用Oct4、Sox2、Klf4、c-Myc 4个转录因子组装在同一表达载体的可切除的慢病毒感染人β-地中海贫血成纤维细胞,建立了5株无饲养层和动物源蛋白的β-地中海贫血iPS细胞系,这些iPS细胞系具有人胚胎干细胞典型的特征,表达人胚胎干细胞的多能性分子标记,如Oct4、Nanog、Tra-1-60等。在体外分化能够形成拟胚体,在体内分化能够形成含有3个胚层类型细胞的畸胎瘤。     

iPS细胞研究的新进展及应用

通过导入特定的转录因子可将分化的体细胞重编程为诱导性多能干细胞(Induced pluripotent stem cells,iPS cells),这项技术避免了干细胞研究领域的免疫排斥和伦理道德问题,是生命科学领域的一次巨大革命。与胚胎干细胞(Embryonic stem cells,ES cells)一样,iPS细胞能够自我更新并维持未分化状态,在体内可分化为3个胚层来源的所有细胞,进而参与形成机体所有组织和器官。在体外,iPS细胞可定向诱导分化出多种成熟细胞。因此,iPS细胞在理论研究和临床应用等方面都极具应用价值。文章对iPS细胞诱导的最新研究进展、iPS细胞诱导的不同方法,如何提高iPS细胞的制备效率和安全性,iPS细胞在基础研究以及临床研究等方面的应用进行了全面综述,并探讨了iPS细胞研究领域面临的问题以及该技术在转基因动物研究中的发展前景。     

致心律失常性右室心肌病患者的诱导性多能干细胞系的建立

目的：建立致心律失常性右室心肌病（ARVC）患者特异性的诱导性多能干细胞（iPSCs）,为研究ARVC发病机制提供研究模型。方法：培养来源于ARVC患者皮肤成纤维细胞,并进行突变位点测序鉴定。通过仙台病毒转导入外源性多能转录因子,将ARVC患者皮肤细胞诱导为iPSCs,结合免疫荧光法,实时荧光定量PCR,以及体内外三胚层形成实验对iPS细胞全能型进行鉴定。通过调控Wnt信号通路诱导iPS细胞定向分化为心肌细胞。结果：ARVC患者来源的iPSCs显示碱性磷酸酶阳性,多能性相关基因高表达,胚胎干细胞标志物Oct4,SSEA4,TRA-1-81阳性。体外悬浮培养形成的拟胚体以及体内畸胎瘤形成实验均显示ARVC-iPSCs具有向3个胚层分化能力。经过体外心肌定向,ARVC-iPSC可诱导产生自主节律性搏动细胞团,免疫荧光显示cTnT阳性。结论：本研究使用仙台病毒,建立了无插入型ARVC患者特异的诱导性多能干细胞系,该细胞系具有多能分化特性,并可定向分化为心肌细胞,为研究ARVC的致病因素和药物筛选提供宝贵的实验模型。     

肝癌细胞系中Yamanaka因子的内源和异位表达及其作用

目的检测肝癌细胞系中Yamanaka因子的表达,为肝癌细胞来源的诱导多能干细胞（iPS细胞）的建立和通过细胞重编程逆转肝癌的恶性表型提供实验依据。方法通过反转录PCR检测Huh7、SMMC-7721、HepG2等肝癌细胞系中4种Yamanaka因子Oct3／4、Sox2、Klf4和c-Myc的mRNA水平,通过Western印迹方法检测上述因子在蛋白质水平的表达,并构建上述因子的慢病毒表达载体,在肝癌细胞中过表达上述转录因子。结果4种Yamanaka因子在肝癌细胞系中均有不同程度表达,mRNA和蛋白质水平的检测结果一致。统计学分析显示,c-Myc的表达显著高于正常肝细胞。成功构建了Yamanaka因子的慢病毒表达载体,并诱导肝癌细胞呈现类似iPS细胞的形态。结论Yamanaka因子在肝癌细胞中有不同程度的内源表达,而外源高表达外源Yamanaka因子对于iPS细胞的诱导至关重要。     

新物种诱导多能干细胞的研究进展

胚胎干细胞（embryonic stem cells,ESC）在人类遗传病学研究、疾病模型建立、器官再生以及动物物种改良和定向变异等方面的地位是其他类型的细胞不可取代的。但是,由于实验技术和体外培养条件的限制,除了小鼠、恒河猴和人之外,大鼠、猪、牛、羊等其他哺乳动物的ES细胞系被证明很难获得。先后有多个研究小组报道了他们利用新兴的诱导多能干细胞（induced pluripotent stem cells,iPS细胞）技术成功建立大鼠和猪的iPS细胞系的研究成果。迄今为止,这两个物种是在未成功建立ES细胞系之前利用iPS技术建立多能干细胞系的成功范例。这些研究对于那些还未建立ES细胞的物种建立多能干细胞系提供了一种新的方案,也将给这些物种的胚胎干细胞的建立、基因修饰动物的产生以及人类医疗事业的促进和发展带来新的希望。     

iPS在临床应用的新进展

诱导性多潜能干细胞,即iPS细胞,是近年来干细胞领域最令人瞩目的一项新的干细胞制造技术,这个技术通过特定的基因组合与转染可以将已分化的体细胞诱导重编程为未分化的多能细胞.与胚胎干细胞(ES)不同,iPS细胞的制造不需要胚胎组织,也不涉及伦理学问题,更重要的是制备iPS细胞可以采用病人自己的体细胞制备,避免免疫排斥反应,并且来源广泛,因此给再生医学实践于临床带来了新的曙光.目前,iPS的研究尚处于初级阶段,本文就iPS的研究现状与已有在临床应用相关的实验报道作以综述.     

肿瘤干细胞及肝癌肿瘤干细胞

肿瘤干细胞理论认为只有存在于肿瘤中的少量干细胞性质的细胞群体对肿瘤发生和发展起着决定作用,肿瘤是由干细胞突变积累而形成的无限增殖的异常组织,这一理论的提出使人们对肿瘤发生机制的认识上升到了一个新的高度,也引起了研究者的广泛关注;肝癌是我国常见的恶性肿瘤之一,我国肝癌死亡率居世界之首,目前对肝癌的研究是我国恶性肿瘤防治的重点工作,现对当前肿瘤干细胞与肝癌肿瘤干细胞相关方面的最新研究进展作一概述。     

Fusion of Tumour Cells with Host Cells

THE A9 cell is an 8-azaguanine-resistant derivative of the L cell line¹. It lacks the enzyme inosinic acid pyrophosphorylase and is thus unable to grow in media such as HAT² in which endogenous synthesis of nucleic acid is blocked by aminopterin. The A9 line has little ability to grow progressively in vivo. Inocula of 5 × 10⁴ to 2 × 10⁶ cells produced progressive tumours in only 12% of X-irradiated newborn syngeneic C3H mice³. One of these tumours was explanted as a cell suspension into Eagle's minimal essential medium containing 15% foetal calf serum and then subcultivated in this medium with 5% foetal calf serum. At each passage, cells were inoculated into X-irradiated newborn syngeneic C3H or semi-allogeneic C3H×X F₁ mice (X designates a number of different allogeneic parents). Between 80 and 90% of the inoculated animals developed progressive tumours. The cell line was therefore designated A9HT (high take incidence). The karyotype of the A9HT line was found to be similar to that of the A9 line, but with a slightly reduced total chromosome number. The modal chromosome number of A9HT was about 53, compared with about 57 for A9 (see ref. 4). A9 and A9HT both had between 20 and 30 bi-armed chromosomes and a number of marker chromosomes in common. A detailed comparison of the karyotypes of the two lines examined by the quinacrine fluorescence technique has been made⁵. The A9HT line, like its A9 parent, lacks inosinic acid pyrophos-phorylase and is unable to grow in HAT medium.     

Dendritic Cells and Regulatory T Cells in Atherosclerosis

Although macrophages and other immune system cells, especially T cells, have been shown to play disease-promoting roles in atherosclerosis, less is known about the role of antigen presenting cells. Functional, immune stimulating dendritic cells (DCs) have recently been detected in aortic intima, the site of origin of atherosclerosis. We had compared DCs with macrophages in mice with experimental atherosclerosis, to clearly define cell types by developmental and functional criteria. This review summarizes recent advances in studies of DCs in humans and in mouse models of atherosclerosis, as well as providing a simple strategy to measure regulatory T (Treg) cells in the mouse aorta.     

Place Cells,Grid Cells,and Memory

The hippocampal system is critical for storage and retrieval of declarative memories, including memories for locations and events that take place at those locations. Spatial memories place high demands on capacity. Memories must be distinct to be recalled without interference and encoding must be fast. Recent studies have indicated that hippocampal networks allow for fast storage of large quantities of uncorrelated spatial information. The aim of the this article is to review and discuss some of this work, taking as a starting point the discovery of multiple functionally specialized cell types of the hippocampal–entorhinal circuit, such as place, grid, and border cells. We will show that grid cells provide the hippocampus with a metric, as well as a putative mechanism for decorrelation of representations, that the formation of environment-specific place maps depends on mechanisms for long-term plasticity in the hippocampus, and that long-term spatiotemporal memory storage may depend on offline consolidation processes related to sharp-wave ripple activity in the hippocampus. The multitude of representations generated through interactions between a variety of functionally specialized cell types in the entorhinal–hippocampal circuit may be at the heart of the mechanism for declarative memory formation.The scientific study of human memory started with Herman Ebbinghaus, who initiated the quantitative investigation of associative memory processes as they take place (Ebbinghaus 1885). Ebbinghaus described the conditions that influence memory formation and he determined several basic principles of encoding and recall, such as the law of frequency and the effect of time on forgetting. With Ebbinghaus, higher mental functions were brought to the laboratory. In parallel with the human learning tradition that Ebbinghaus started, a new generation of experimental psychologists described the laws of associative learning in animals. With behaviorists like Pavlov, Watson, Hull, Skinner, and Tolman, a rigorous program for identifying the laws of animal learning was initiated. By the middle of the 20th century, a language for associative learning processes had been developed, and many of the fundamental relationships between environment and behavior had been described. What was completely missing, though, was an understanding of the neural activity underlying the formation of the memory. The behaviorists had deliberately shied away from physiological explanations because of the intangible nature of neural activity at that time.Then the climate began to change. Karl Lashley had shown that lesions in the cerebral cortex had predictable effects on behavior in animals (Lashley 1929, 1950), and Donald Hebb introduced concepts and ideas to account for complex brain functions at the neural circuit level, many of which have retained a place in modern neuroscience (Hebb 1949). Both Lashley and Hebb searched for the engram, but they found no specific locus for it. A significant turning point was reached when Scoville and Milner (1957) reported severe loss of memory in an epileptic patient, patient H.M., after bilateral surgical removal of the hippocampal formation and the surrounding medial temporal lobe areas. “After operation this young man could no longer recognize the hospital staff nor find his way to the bathroom, and he seemed to recall nothing of the day-to-day events of his hospital life.” This tragic misfortune inspired decades of research on the function of the hippocampus in memory. H.M.’s memory impairment could be reproduced in memory tasks in animals and studies of H.M., as well as laboratory animals, pointed to a critical role for the hippocampus in declarative memory—memory, which, in humans, can be consciously recalled and declared, such as memories of experiences and facts (Milner et al. 1968; Mishkin 1978; Cohen and Squire 1980; Squire 1992; Corkin 2002). What was missing from these early studies, however, was a way to address the neuronal mechanisms that led information to be stored as memory.The aim of this article is to show how studies of hippocampal neuronal activity during the past few decades have brought us to a point at which a mechanistic basis of memory formation is beginning to surface. An early landmark in this series of investigations was the discovery of place cells, cells that fire selectively at one or few locations in the environment. At first, these cells seemed to be part of the animal’s instantaneous representation of location, independent of memory, but gradually, over the course of several decades, it has become clear that place cells express current as well as past and future locations. In many ways, place cells can be used as readouts of the memories that are stored in the hippocampus. More recent work has also shown that place cells are part of a wider network of spatially modulated neurons, including grid, border, and head direction cells, each with distinct roles in the representation of space and spatial memory. In this article, we shall discuss potential mechanisms by which these cell types, particularly place and grid cells, in conjunction with synaptic plasticity, may form the basis of a mammalian system for fast high-capacity declarative memory.     

体细胞重编程逆转为干细胞的研究进展

目前细胞和发育生物学上的研究成果为生物医学研究提供了广泛的前景.将完全分化的细胞重编程,不经过胚胎逆转为多能干细胞状态,这点燃了再生医学应用的新希望,这一成果从法律、道德、伦理等不同方面被人们所接受.通过体细胞克隆胚胎获得干细胞所面临的破坏胚胎的伦理限制,促使研究者去寻求将分化细胞重编程逆转为干细胞的新方法.主要论述了体细胞重编程的原理、过程及不经过胚胎逆转为多能干细胞的方法.     

Dendritic Cells: Migratory Cells that are Attractive

Dendritic cells (DC) are professional antigen presenting cells, playing an important role in the initiation of T- and T cell dependent immune responses. DC are highly mobile cells and the sequential migration of DC in and out of tissues is accompanied by phenotypical as well as functional changes instrumental to their function as sentinels of the immune system. Herein, we will review recent progress in understanding the origin of DC, their migratory behaviour and their capacity to attract and interact with lymphocytes, with emphasis on the chemokine system.     

IDS Transfer from Overexpressing Cells to IDS-Deficient Cells

Iduronate sulfatase (IDS) is responsible for mucopolysaccharidosis type II, a rare recessive X-linked lysosomal storage disease. The aim of this work was to test the ability of overexpressing cells to transfer IDS to deficient cells. In the first part of our work, IDS processing steps were compared in fibroblasts, COS cells, and lymphoblastoid cell lines and shown to be identical: the two precursor forms (76 and 90 kDa) were processed by a series of intermediate forms to the 55- and 45-kDa mature polypeptides. Then IDS transfer to IDS-deficient cells was tested either by incubation with cell-free medium of overexpressing cells or by coculture. Endocytosis and coculture experiments between transfected Lβ and deleted fibroblasts showed that IDS transfer occurred preferentially by cell-to-cell contact as IDS precursors are poorly secreted by transfected Lβ. The 76- and 62-kDa IDS polypeptides transferred to deleted fibroblasts were correctly processed to the mature 55- and 45-kDa forms. Lβ were not able to internalize the 90-kDa phosphorylated precursor forms excreted in large amounts in the medium of overexpressing fibroblasts. Enzyme transfer occurred only by cell-to-cell contact, but the precursor forms transferred in Lβ after cell-to-cell contact were not processed. This absence of maturation was probably due to a mistargeting of IDS precursors in these cells.     

Oocyte-like Cells Induced from Mouse Spermatogonial Stem Cells

ABSTRACT: BACKGROUND: During normal development primordial germ cells (PGCs) derived from the epiblast are the precursors of spermatogonia and oogonia. In culture, PGCs can be induced to dedifferentiate to pluripotent embryonic germ (EG) cells in the presence of various growth factors. Several recent studies have now demonstrated that spermatogonial stem cells (SSCs) can also revert back to pluripotency as embryonic stem (ES)-like cells under certain culture conditions. However, the potential dedifferentiation of SSCs into PGCs or the potential generation of oocytes from SSCs has not been demonstrated before. RESULTS: We report that mouse male SSCs can be converted into oocyte-like cells in culture. These SSCs-derived oocytes (SSC-Oocs) were similar in size to normal mouse mature oocytes. They expressed oocyte-specific markers and give rise to embryos through parthenogenesis. Interestingly, the Y- and X-linked testis-specific genes in these SSC-Oocs were significantly down-regulated or turned off, while oocyte-specific X-linked genes were activated. The gene expression profile appeared to switch to that of the oocyte across the X chromosome. Furthermore, these oocyte-like cells lost paternal imprinting but acquired maternal imprinting. CONCLUSIONS: Our data demonstrate that SSCs might maintain the potential to be reprogrammed into oocytes with corresponding epigenetic reversals. This study provides not only further evidence for the remarkable plasticity of SSCs but also a potential system for dissecting molecular and epigenetic regulations in germ cell fate determination and imprinting establishment during gametogenesis.