El ácido all trans retinoico reduce in vitro el efecto protumoral de los factores de crecimiento e incrementa la eficacia de la quimioterapia en el rabdomiosarcoma S4MH

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Estudio de los sueros ricos en factores de crecimiento y de su efecto sobre células de epitelio corneal

Objetivos: Estudiar cómo afecta a la concentración de determinados factores de crecimiento presentes en los sueros la filtración (utilizado como método de esterilización) y el tratamiento por calor (utilizado para la inactivación del complemento). Además de estudiar el efecto de un bioadhesivo (ácido hialurónico, HaNa), aplicado solo o conjuntamente con el suero rico en factores de crecimiento (s-PRGF), sobre la capacidad de las células de epitelio corneal (HCE) para proliferar y migrar. Materiales y métodos: Se midió mediante kits ELISA comerciales la concentración en las diferentes condiciones de filtración y calentamiento de las siguientes biomoléculas EGF (Epidermal Growth Factor), VEGF (Vascular Endothelial Growth Factor), HGF (Hepatocyte Growth Factor), PDGF (Platelet-derived Growth Factor) y la Fibronectina. Teniendo en cuenta el papel de la proliferación y migración celular en los procesos de cicatrización se han realizado dos ensayos diferentes in vitro: un ensayo MTT para estudiar la viabilidad y la proliferación celular y el método de la herida (Scratch wound-healing assay) para determinar la capacidad migratoria de células bajo ciertos tratamientos: BSA (Bovine Serum Albumin) al 1% como control, FBS (Fetal Bovine Serum) al 10%, s-PRGF al 45%, s-PRGF al 45% con HaNa 0,1% y HaNa al 0,1% Resultados: En el caso de la filtración, se observa una mayor pérdida de factores utilizando un filtro con una membrana de PVDF (Durapore®) para todos los factores estudiados. El calentamiento produce una reducción de la concentración superior al 50% en el caso del HGF y EGF, manteniéndose constante en el caso del VEGF.La mezcla de diferentes muestras con el complemento inactivado para formar un pool no presenta cambios en la concentración al compararlo con la media de las muestras utilizadas. Por tanto, la utilización de un pool del hemoderivado no supone perdida de factores de crecimiento, haciendo de ello un procedimiento perfectamente aceptable para los ensayos celulares. El tratamiento con s-PRGF y el combinado con el bioadhesivo promueven la proliferación y migración de las células de epitelio corneal humano(HCE) in vitro de manera similar, no encontrándose diferencias estadísticamente significativas entre ambos. Conclusiones: La adicción del bioadhesivo no produce efecto tóxico en las células, sin embargo, no se han encontrado efectos beneficiosos en cuanto a proliferación y migración se refiere. A este respecto, creemos que hay que dar un paso más haciendo comprobaciones in vivo, ya que, a diferencia de la experimentación in vitro los componentes de los hemoderivados no están indefinidamente en contacto con las células sino por un espacio de tiempo muy reducido. Por ello, la concentración de factores de crecimiento en la aplicación in vivo es especialmente importante, y no sería conveniente reducirla mediante procedimientos físicos como la filtración o el calentamiento.

树鼩肝细胞体外分离培养体系的复建及主要影响因素分析

树鼩(Tupaia Belangeri)与人和灵长类亲缘关系较为接近,是乙型肝炎研究中备受关注的小动物模型,而其原代肝细胞的分离和培养则足建立HBV体外感染模型及应用和基础研究的关键的第一步,但由于以往的文献报道均较为简要,需要较长时间的摸索.本研究通过与机械分离法的直接比较,验证了两步灌注法在树鼩肝细胞分离中的优越性.进而发现,在分离后的体外培养过程中,二甲基亚砜不仪能够促进和维持原代肝细胞的分化,而且能够显著地抑制纤维状细胞群的出现.同时,肝细胞生长因子(HGF)和表皮生长因子(EGF)能够促进肝细胞在体外长期存活.在此优化的条件下,原代培养可持续4-5周,并且较多的细胞聚集形成类似肝窦结构的形态,从而为乙型肝炎病毒感染机理研究和药物筛选提供了必备的先决条件,也为内型肝炎病毒和丁型肝炎病毒及单纯疱疹病毒等研究和药物筛选提供了可能.

Transplantable neural progenitor populations derived from Rhesus monkey embryonic stem cells

Cell-based therapies using embryonic stem cells (ESCs) in the treatment of neural disease will require the generation of homogenous donor neural progenitor (NP) populations. Here we describe an efficient culture system containing hepatocyte growth factor (HGF) and G5 supplement for the production of highly enriched (88.3% +/- 8.1%)populations of NPs from rhesus monkey ESCs. Additional purification resulted in NP preparations that were 98% nestin positive. Moreover, NPs, as monolayers or neurospheres, could be maintained for prolonged periods of time in media containing HGF+G5 or G5 alone. In vitro differentiation and in vivo transplantation assays showed that NPs could differentiate into neurons, astrocytes, and oligodendrocytes. The kinds and quantities of differentiated cells derived from NPs were closely correlated with their niches in vivo. Glial differentiation was predominant in periventricular areas, whereas cells migrating into the cortex were mostly neurons. Cell counts showed that 2 months after transplantation, approximately 25% of transplanted NPs survived and 65% - 80% of the surviving transplanted cells migrated along the ventricular wall or in a radial fashion. Subcloning demonstrated that several clonal lines derived from NPs expressed nestin and differentiated into three neural lineages in vitro and in rat brains in vivo. In contrast, some subcloned lines showed restricted differentiation both in vitro and in vivo in rat brains. These observations set the stage for obtaining highly enriched NPs and evaluating the efficacy of NP-based transplantation therapy in the nonhuman primate and will provide a platform for probing the molecular mechanisms that control neural induction.

Neural progenitors derived from monkey embryonic stem cells in a simple monoculture system

A simple monoculture system. combined with a chemically defined medium containing hepatocyte growth factor (HGF) and G5 supplement, was used to induce rhesus monkey embryonic stem cells (rESC) directly into neuroepithelial (NE) cells. Under these conditio

肝细胞生长因子促进猕猴胚胎干细胞来源的神经前体细胞的增殖

肝细胞生长因子（HGF）是一个多效应因子，在神经系统中具有重要作用， 但是对于HGF在早期神经系统发育（特别是哺乳动物）中的具体作用还不明确， 这方面的研究还很少。我们早前的研究发现采用HGF和G5 supplement结合EB法 可诱导猕猴胚胎干细胞（rESCs）定向分化成高纯度（88.3± 8.1%）的可移植的 神经前体细胞，但是HGF在整个分化过程中的具体作用及HGF与其它因子的关 系还不清楚。 本研究改进先前研究体系，用单层培养诱导体系代替EB法诱导体系，用bFGF 代替G5 supplement。即采用单层培养的方式，分别用同时含bFGF和HGF、只含 HGF或bFGF以及两者都没有添加的成分确定的分化液诱导rESCs向神经细胞分 化。并检测HGF对rESCs来源的神经前体细胞的增殖速度的影响，旨在进一步研 究HGF在整个分化过程中的具体作用及HGF与bFGF的关系。主要结论如下：1） 采用单层培养法，同时添加HGF和bFGF可诱导rESCs在两周内定向分化为高纯度 （>85%）的神经前体细胞，从而建立了一种更为简单的诱导rESCs分化成神经细 胞的方法；2）不同分化条件下都得到了相似比例的神经前体细胞，表明外源性 的HGF在诱导rESC向神经前体细胞转变的过程中对于神经细胞命运的决定并不 起作用；3）HGF能有效地促进rESCs来源的神经前体细胞的增殖，并且与bFGF 具有协同作用。

肝细胞生长因子促进猕猴胚胎干细胞来源的神经前体细胞的增殖

肝细胞牛长因子(hepatoeyte growth factor,HGF)足一个多效应因子,在神经系统中具有重要作用.早前的研究发现采用HGF和G5 supplement结合EB(embryoid body)法可诱导猕猴胍胎干细胞(rhesus embryonic stem cells,rESCs)定向分化成高纯度的可移植的神经前体细胞(neural progenitors),但对于HGF在整个诱导分化过程中的具体作用及机制还不清楚.本研究改进先前研究体系,采用单层培养法,同时添加HGF和bFGF(basic fibroblast growth factor,碱性成纤维细胞生长因子)诱导rESCs在两周内定向分化为高纯度[(81.66±4.37)%]的神经前体细胞,并且单独添加HGF或bFGF以及两者都没有添加的条件下也得到了相似比例的神经前体细胞,表明外源性的HGF在诱导rESCs向神经前体细胞转变的过程中对十神经细胞命运的决定并不起作用;进一步研究发现HGF能有效地促进神经前体细胞的增殖,并且与bFGF具有协同作用.总之,本研究建立了一种更为简单的诱导rESCs分化成神经细胞的方法,发现外源性的HGF在rESCs向神经前体细胞分化的过程中并没有神经诱导的作用,但能与bFGF协同作用促进rESCs来源的神经前体细胞的增殖.

Hepatocyte growth factor enhances the generation of high-purity oligodendrocytes from human embryonic stem cells

Generation of homogeneous oligodendrocytes as donor cells is essential for human embryonic stem cell (hESC)-based cell therapy for demylinating diseases. Herein we present a novel method for efficiently obtaining mature oligodendrocytes from hESCs with high purity (79.7 +/- 6.9%), using hepatocyte growth factor (HGF) and G5 supplement(containing insulin, transferrin, selenite, biotin, hydrocortisone, basic fibroblast growth factor and epidermal growth factor) in a four-step method. We induced hESCs into neural progenitors (NP) with HGF (5 ng/ml) and G5 (1 x) supplemented medium in an adherent differentiation system. The purified NPs were amplified in suspension as neurospheres for 1 month, and terminal oligodendrocyte differentiation was then induced by G5 supplement withdrawal and HGF treatment (20 ng/ml). The cells generated displayed typical morphologies of mature oligodendrocytes and expressed oligodendrocyte markers O4 and myelin basic protein (MBP). Our result revealed that HGF significantly enhanced the proliferation of hESC-derived NPs and promoted the differentiation as well as the maturation of oligodendrocytes from NPs. Further studies suggest that HGF/c-Met signaling pathway might play an important role in oligodendrocyte differentiation in our system. Our studies provide a means for generating the clinically relevant cell type and a platform for deciphering the molecular mechanisms that control oligodendrocyte differentiation. (C) 2009 International Society of Differentiation. Published by Elsevier Ltd. All rights reserved.

树鼩原代肝细胞培养体系和乙型肝炎病毒体外感染模型的建立

乙型肝炎病毒（Hepatitis Virus type B, HBV）感染是一种严重威胁人类健康的世界性问题。由于HBV感染具有宿主和组织特异性，长期以来一直缺乏有效的体外感染模型，严重制约了HBV感染机制和治疗药物的研究。树鼩（Tree Shrews, Tupaia Belangeri）与人和灵长类亲缘关系较为接近，作为小动物模型在乙型肝炎研究中备受关注。但由于各种原因的限制，HBV树鼩感染模型仍处于“国际公认但实际短缺，国内首创但实际空缺”的状况。因此，复建和优化HBV树鼩体内外感染模型成为我们长期研究方向所必备的前提基础和开端。而树鼩原代肝细胞的分离和培养则是建立HBV体外感染模型的关键的第一步。我们通过与机械分离法的直接比较，验证了两步灌注法在树鼩肝细胞分离中的优越性。进而发现，在分离后的体外培养过程中，二甲基亚砜不仅能够促进和维持原代肝细胞的分化，而且能够显著地抑制纤维状细胞群的出现。同时，肝细胞生长因子（HGF）和表皮生长因子（EGF）能够促进肝细胞在体外长期存活。在此优化的条件下，原代培养可持续4-5周，并且较多的细胞聚集形成类似肝窦结构的形态，从而成功地复制和改进了树鼩原代肝细胞培养体系，为建立HBV体外感染模型提供了基础。与此同时，我们采集了2种来源的HBV，即以乙肝病人血清和HepG2.2.15细胞培养上清为来源。我们采用蔗糖浓度梯度离心法以纯化病人血清病毒，能较好地将HBV颗粒和亚病毒颗粒区分开来。在收集HepG2.2.15细胞株来源的病毒时，我们详细研究了HepG2.2.15细胞的生长曲线和病毒产量曲线，找到病毒产量与细胞生长状态之间的联系，确定了最佳收集病毒时间，并通过放大培养条件，大量收集HepG2.2.15细胞的培养上清。我们采用浓缩和未浓缩的HepG2.2.15病毒、纯化的血清病毒等3种方式制备的病毒感染树鼩原代肝细胞，通过不同水平的指标来检测感染结果。首先，细胞内HBVx基因mRNA的检测结果表明，3种来源的病毒都可以感染树鼩原代肝细胞。同时，细胞上清中分泌的病毒颗粒及病毒蛋白的检测结果表明，HepG2.2.15病毒感染树鼩原代肝细胞的效果比血清病毒的感染效果好。免疫荧光的检测结果进一步证实了HepG2.2.15病毒能够感染树鼩原代肝细胞。因此，在我们的实验中，树鼩原代肝细胞对2种来源和不同制备方式的病毒均具有易感性，且以未浓缩的HepG2.2.15上清病毒感染力优于血清病毒。综上所述，我们现有的结果验证了树鼩原代肝细胞对HBV具有易感性。就感染效率而言，尽管感染效率依赖于病毒滴度及其感染力，我们在病毒细胞比例为0.02:1的条件下，仍能确认易感性，并获得了与国际同类研究相当的感染效率。就本研究的应用前景而言，我们所建立的HBV体外感染模型，能够作为实验室的通用平台，用以来研究HBV的感染机制和抗病毒药物的筛选与评价。

猕猴多潜能成体肝前体细胞及猕猴ES 定向分化为胆管上皮细胞的研究

为解决供体器官的不足，以细胞移植为基础的替代疗法已成为治疗不可逆肝 脏疾病新的希望。 肝前体（干）细胞（Hepatic progenitor cellS，HPCs）和 胚胎干细胞（embryoic stem cells, ES）由于其特殊的细胞特性已成为细胞替 代治疗理想的种源细胞。 然而一方面包括人在内的灵长类动物的正常成体肝来 源的HPCs 的分离依然是很困难的；另一方面，ES 细胞来源的肝细胞和胆管细胞 的生成效率依旧很低。因此有必要建立稳定的高效的灵长类动物HPCs 细胞分离 培养体系及ES 细胞的肝细胞或胆管细胞分化体系以满足供体细胞的不足；这种 体系的建立还有利于研究肝细胞生物学如分化机制、自我更新机制等方面的重要 基础问题。 本研究以猕猴为实验模型，研究了正常成体肝来源的猕猴HPCs 分离、纯化 的条件，系统地鉴定了猕猴HPCs 的细胞特性和体内、外分化潜能，并评价了体 内移植效果。 同时以rES 为材料，建立了rES 高效分化为限定性内胚层 （definitive endoderm cells, DE）和胆管上皮细胞的分化体系。主要实验结 果包括：1）： FBS、EGF、HGF 及rat tail collagen (鼠尾胶原)是分离培养正 常成体猕猴来源的肝上皮前体细胞(rhesus monkey liver epithelial progenitor cells, mLEPCs)所必需的，mLEPCs 在此培养体系中至少可以扩增20 代或5 个月以上，并仍然保持原有的细胞特性；mLEPCs 呈现典型的上皮细胞形 态，并表达HPCs 细胞特有的表达模式即同时表达肝细胞和胆管细胞相关基因 （ALB，APOH，CX43，IB4）或蛋白（CK7，CK8，CK18）；在适宜的分化体系下， mLEPCs 可分化为功能性的肝细胞，形成具有胆管上皮细胞的胆管样结构，并能 转分化形成肌肉样细胞、肌样成纤维细胞及少突样细胞；移植入肝损伤的免疫抑 制的小鼠体内后，mLEPCs 能参与受体肝组织的再生，并能分化成ALB 阳性的肝 细胞；体内定位发现mLEPCs 与胆管区的细胞有相似的免疫原性，提示mLEPCs 可能来源于胆管区。2）：rES 在高浓度的acitvin A（100ng/ml）和低浓度的血 清(1%)单层诱导体系下可定向分化得到高比率的限定性内胚层细胞（definitive endoderm cells，DE 细胞）(约80%)； 高比率的DE 细胞的得到还与rES 细胞的接种密度相关；BMP4 和FGF1 可诱导DE 细胞高效向胆管上皮细胞分化（约90%）， 但并不能得到肝细胞；而Notch 信号通路可维持DE 细胞的存活，并决定着DE 细胞向胆管细胞分化，在Notch 信号通路失活的情形下，即使存在BMP4 和FGF1 都不能促使DE 细胞向胆管细胞分化。 本实验首次成功建立了正常猕猴成体肝HPCs 分离培养体系，证实了分离得 到的猕猴肝上皮前体细胞不但具有正常HPCs 的增殖活力和参与受体肝组织的再 生能力，而且还具有三个胚层的分化潜能，这一结果将为以HPCs 为基础的细胞 替代治疗人类肝脏疾病的实现提供了可能，并首次证明了HPCs 也可以像某些少 数成体干细胞一样具有三个胚层得分化潜能。 此外，本研究建立了rES 高效定 向分化为DE 细胞和胆管细胞的分化体系，这一方法的建立将促进灵长类动物的 DE 细胞的发育机制研究，同时也可为高比率的内胚层功能细胞（如胰岛细胞、 肝细胞、肺细胞）的获得提供丰富的种源细胞和平台。

人胚胎干细胞建系及向神经细胞定向分化的研究

研究和利用人胚胎干细胞(hES)细胞已成为生命科学领域的核心问题之一。当前hES 细胞研究主要集中在hES 的建系和维持其不分化状态；提高hES 细胞定向分化为特定 细胞的比例；ES 细胞自我更新和分化的机制等方面。本论文一方面概述了hES 细胞相 关领域的研究进展；另一方面建立了不同培养体系条件下3 株hES 细胞，并在此基础 上利用G5 和肝生长因子（HGF）诱导hES 细胞定向分化成高纯度的NPs。主要结论如 下：1) 建立人卵体外受精和胚胎培养体系。获得了15 个囊胚，采用了免疫外科法分离 内细胞团，运用含血清以及不含血清的培养体系，在ICR 小鼠胚胎成纤维饲养层上分 别建立了YKh-1、YKh-2 和YKh-3 3 株人胚胎干细胞系，生长良好，核型正常。ES 细 胞表达碱性磷酸酶活性、SSEA-3、SSEA-4、TRA-1-60、TRA-1-81 和Oct-4，但不表达 SSEA-1； ES 细胞在体外能够分化为属于外胚层、中胚层和内胚层的各种分化细胞， 在SCID 小鼠体内能形成畸胎瘤，畸胎瘤包括了所有三个胚层来源的细胞类型。证实了 ES 细胞系的多向分化潜能。2) 对比含血清以及无血清的培养体系的hES 细胞系的特征， 观察了其集落形态、生长速度、分化能力。结果表明，在含血清培养体系的Yhk-2，其 集落形态较致密，含2-3 个核的细胞较多，细胞倍增时间为43.9±5.7h；而在无血清培 养体系的Yhk-3，其集落形态较铺展，细胞较小而圆，倍增时间为34.8±3.8h。细胞免疫 染色和PCR 结果表明，二者在体外都能分化为三个胚层来源的多种细胞，但比例有所 差异。提示二者在向三个胚层来源的细胞的分化能力上有所不同。 3) 以所建立的hES 细胞系为模型，采用HGF 和G5 作为诱导因子添加到神经诱导培养基中，诱导hES 细 胞分化成高纯度的NPs。单独的HGF 或G5 仅能诱导ES 细胞分化成70.9± 5.0%和 72.9±7.2%NPs，而联用HGF 和G5 使NPs 的比率达到91.2±11.2%，进一步纯化后获得 98±3.2%的NPs。获得的NPs 能分化成三个谱系神经细胞，亚克隆实验也进一步证明采 用HGF+G5 获得的单个NPs 具有神经干细胞的特性，也能在体外分化成三个谱系的神 经细胞。用SHH 处理NPs，获得的分化细胞表达不同脑区标志，表明所得到NPs 具有 对脑区信号发生反应，进一步分化为不同脑区神经元细胞的能力。 本实验建立了具有自主知识产权的中国人源胚胎干细胞系，建立了ES 细胞的含血 清以及无血清的培养体系和向神经前体细胞定向分化系统，得到高比例的神经前体细 胞，为进一步研究利用人胚胎干细胞打下良好的基础。

猕猴胚胎干细胞培养以及定向分化成神经细胞的研究

灵长类胚胎干细胞（Es）的研究不仅对理解生殖发育生物学的基础理论、而且对实现细胞替代治疗具有重要意义。当前灵长类ES细胞还有很多问题需要解决，如ES细胞培养体系的改进、ES细胞定向分化成高纯度特定组织细胞的可能性、有效性以及分化机制等问题。本文一方面概述了灵长类ES细胞相关领域的研究进展；另一方面，以称猴胚胎干细胞（rEs）为材料，在改善rES细胞的培养体系、提高其定向分化成神经前体细胞（NPs）和少突细胞的比率进行了研究。实验采用同源称猴细胞系作为饲养层培养rES细胞，并在此基础上利用肝生长因子（HGF）和GS诱导rES细胞定向分化成高纯度的NPs和少突细胞，并评价了NPs是否具有移植功能。主要结论如下：1）四种称猴细胞系（MOF、MESF、MFG和CMESF）可作为饲养层支持rES细胞的生长，保持ES自我更新的能力和分化的多能性。而且这几种称猴饲养层支持ES细胞生长的能力存在明显的差异，进一步的研究表明这些差异主要是由于基因表达种类以及表达量上的差异而导致的。2）采用HGF和GS作为诱导因子添加到NDCM液中，诱导rES细胞分化成可移植的NPs。实验结果如下：单独的HGF或GS仅能诱导ES细胞分化成65±8.3％和69±14％NPs，而HGF和GS的联合使用NPs的比率达到88.3±8.1％，进一步纯化后获得98±1.2％的NPs。获得的NPs能在体内、外分化成三个谱系神经细胞，并能整合到大鼠脑部，发生迁移和分化。25％的NPs细胞8周后仍保持存活状态，其中65-80％的细胞发生了不同程度的迁移，而且细胞在脑部的分化种类以及数目与细胞在体内所处的微环境具有重要的关系。亚克隆实验也进一步证明采用HGF＋GS获得的部分单个NPs具有神经干细胞的特性，也能在体内、外分化成三个谱系的神经细胞，而另外的却只能分化成其中的一、两种谱系的细胞。3）利用五步法，ES细胞能分化成75±6.8％的少突祖细胞和81土8．6％的成熟少突细胞。HGF通过抑制NPs的凋亡和缩短NPs的复制周期，共同促进NPs的增殖。HGF也能诱导HGF+G5获得的NPs分化成少突祖细胞和成熟少突细胞，并且促进少突细胞成熟。而且HGF促进NPs分化成少突细胞的能力受到GS的调控，单独HGF作用将导致ES细胞分化成神经元。本实验的结果为促进rES细胞相关领域的研究，以及ES细胞在神经系统疾病临床应用上提供信息，也为研究NPs和少突细胞的发育提供典型的细胞模型。

Immediate early gene expression in dog thyrocytes in response to growth, proliferation, and differentiation stimuli.

In dog thyroid cells, insulin or IGF-1 induces cell growth and is required for the mitogenic action of TSH through cyclic AMP, of EGF, and of phorbol esters. HGF per se stimulates cell proliferation and is thus the only full mitogenic agent. TSH and cAMP enhance, whereas EGF phorbol esters and HGF repress differentiation expression. In this study, we have investigated for each factor and regulatory cascade of the intermediate step of immediate early gene induction, that is, c-myc, c-jun, jun D, jun B, c-fos, fos B, fra-1, fra-2, and egr1; fra-1 and fra-2 expressions were very low. TSH or forskolin increased the levels of c-myc, jun B, jun D, c-fos, and fos B while decreasing those of c-jun and egr1. Phorbol myristate ester stimulated the expression of all the genes. EGF and HGF stimulated the expression of all the genes except jun D and for EGF fos B. All these effects were obtained in the presence and in the absence of insulin, which shows that insulin is not necessary for the effects of the mitogens on immediate early gene expression. The definition of the repertoire of early immediate genes inductible by the various growth cascades provides a framework for the analysis of gene expression in tumors. (1) Insulin was able to induce all the protooncogenes investigated except fos B. This suggests that fos B could be the factor missing for insulin to induce mitogenesis. (2) No characteristic pattern of immediate early gene expression has been observed for insulin, which induces cell hypertrophy and is permissive for the action of the other growth factors. These effects are therefore not accounted for by a specific immediate early gene expression. On the other hand, insulin clearly enhances the effects of TSH, phorbol ester, and EGF on c-myc, junB, and c-fos expression. This suggests that the effect of insulin on mitogenesis might result from quantitative differences in the transcription complexes formed. (3) c-myc, c-fos, and jun B mRNA induction by all stimulating agents, whether inducing cell hypertrophy, or growth and dedifferentiation, or growth and differentiation, suggests that, although these expressions are not sufficient, they may be necessary for the various growth responses of thyroid cells. (4) The inhibition of c-jun and egr1 mRNA expression, and the marked induction of jun D mRNA appear to be specific features of the TSH cAMP pathway. They might be related to its differentiating action. (5) fos B, which is induced by TSH, forskolin, phorbol ester, and HGF but not by insulin, could be involved in the mitogenic action of the former factors.

IGF-1 or insulin, and the TSH cyclic AMP cascade separately control dog and human thyroid cell growth and DNA synthesis, and complement each other in inducing mitogenesis.

The regular doubling of cell mass, and therefore of cell protein content, is required for repetitive cell divisions. Preliminary observations have shown that in dog thyrocytes insulin induces protein accumulation but not DNA synthesis, while TSH does not increase protein accumulation but triggers DNA synthesis in the presence of insulin. We show here that EGF and phorbol myristate ester complement insulin action in the same way. HGF is the only factor activating both protein accumulation and DNA synthesis. The effects of insulin on protein accumulation and in permitting the TSH effect are reproduced by IGF-1 and are mediated, at least in part by the IGF-1 receptor. The concentration effect curves are similar for both effects. Similar results are obtained in human thyrocytes. They reflect true cell growth, as shown by increases in RNA content and cell size. Carbachol and fetal calf serum also stimulate protein synthesis and accumulation without triggering DNA synthesis, but they are not permissive for the mitogenic effects of TSH or of the general adenylate cyclase activator, forskolin. Moreover the mitogenic effect of TSH greatly decreased in cells deprived of insulin for 2 days although these cells remain hypertrophic. Hypertrophy may therefore be necessary for cell division, but it is not sufficient to permit it. Three different mechanisms can therefore be distinguished in the mitogenic action of TSH: (1) the increase of cell mass (hypertrophy) induced by insulin or IGF-1; (2) the permissive effect of insulin or IGF-1 on the mitogenic effect of TSH which may involve both the increase of cell mass and the induction of specific proteins such as cyclin D3 and (3) the mitogenic effect of the TSH cyclic AMP cascade proper.

Association of polymorphisms in the hepatocyte growth factor gene promoter with keratoconus

Purpose. Keratoconus is a progressive disorder of the cornea that can lead to severe visual impairment or blindness. Although several genomic regions have been linked to rare familial forms of keratoconus, no genes have yet been definitively identified for common forms of the disease. Methods. Two genome-wide association scans were undertaken in parallel. The first used pooled DNA from an Australian cohort, followed by typing of top-ranked single-nucleotide polymorphisms (SNPs) in individual DNA samples. The second was conducted in individually genotyped patients, and controls from the USA. Tag SNPs around the hepatocyte growth factor (HGF) gene were typed in three additional replication cohorts. Serum levels of HGF protein in normal individuals were assessed with ELISA and correlated with genotype. Results. The only SNP observed to be associated in both the pooled discovery and primary replication cohort was rs1014091, located upstream of the HGF gene. The nearby SNP rs3735520 was found to be associated in the individually typed discovery cohort (P = 6.1 × 10 ). Genotyping of tag SNPs around HGF revealed association at rs3735520 and rs17501108/rs1014091 in four of the five cohorts. Meta-analysis of all five datasets together yielded suggestive P values for rs3735520 (P = 9.9 × 10 ) and rs17501108 (P = 9.9 × 10 ). In addition, SNP rs3735520 was found to be associated with serum HGF level in normal individuals (P = 0.036). Conclusions. Taken together, these results implicate genetic variation at the HGF locus with keratoconus susceptibility. © 2011 The Association for Research in Vision and Ophthalmology, Inc.