成人胰岛细胞移植25例次临床研究

目的 建立新型成人胰岛细胞分离纯化方法,观察成人胰岛细胞移植的安全性与有效性.方法 对14例1型糖尿病(T1DM)患者进行PFC与UW液双层冷藏胰腺,Liberase酶消化,COBE 2991型专用胰岛细胞分离机分离及连续密度梯度纯化,获取高纯度与高活性的胰岛细胞.采用外科方法,将短期培养的胰岛细胞经门静脉移植到肝脏内...     

鸡胚睾丸支持细胞的分离、纯化与鉴定

以18天鸡胚睾丸为实验材料,经胶原酶和胰蛋白酶两步酶消化法得到生精上皮细胞悬液.在原代培养过程中经差异贴壁和低渗处理后,获得了纯度约为90%的单层支持细胞.对纯化的培养物染色鉴定,结果显示支持细胞为碱性磷酸酶(AKP)阴性,而混杂在其中的另一种体细胞管周细胞为AKP阳性;油红O染色显示,支持细胞胞质内含有大量的脂肪滴,核内见双极小体;吖啶橙染色证实支持细胞富含RNA;罗丹明123染色显示支持细胞富含线粒体;Hoechst 33342染色显示支持细胞细胞核呈长卵圆形,核的长轴与细胞长轴平行;免疫荧光染色显示支持细胞胞质中表达波形蛋白.建立了一套简单、易行的鸡胚睾丸支持细胞分离纯化与鉴定方法.     

胰岛细胞与供者抗原特异性调节性T细胞共移植

胰岛移植是治疗1型糖尿病（ Type 1 diabetes, T1DM）的一种很有前途的方法。近年来按照 Edmond 方案进行的移植,已大大提高了1年不依赖胰岛素率,但远期疗效仍然很低[1]。即使在目前全球效果最好的加拿大？Edmonton？Alberta？大学,其5年不依赖胰岛素率也只有8.5﹪[2]。远期疗效欠佳的重要原因之一便是成功的胰岛移植除了要克服同种排斥反应外,还必须控制糖尿病个体的自身免疫损伤[3],这与心脏、肝脏和肾脏等其它脏器移植是绝然不同的。     

睾丸支持细胞紧密连接的动力学调控

在睾丸精子发生的过程中,处于细线期和细线前期的精母细胞必须从生精上皮的基底室进入近腔室,这样形态上发育完全的精子才能在精子释放时进入到生精小管的内腔。显然,构成血-睾屏障的支持细胞间紧密连接的开放和关闭受到一系列信号分子的调节。已经发现的对该过程起调控作用的信号分子包括：转化生长因子β3(TGFβ3)、闭锁蛋白、PKA、PKC等。现就该领域研究的新进展以及可用于研究紧密连接动力学的一些模型进行综述。     

牛睾丸支持细胞分离、纯化及体外生长行为的研究

了解牛睾丸支持细胞体外培养的生物学特性,试验采用组合酶消化和选择贴壁法,将5月龄、6月龄牛胎儿及新生牛睾丸支持细胞分离纯化后进行体外培养。试验结果显示,这一阶段牛睾丸适宜支持细胞分离纯化用;采用0.25 %胰蛋白酶+0.02 %EDTA二次消化法是一种经济有效的牛胎儿睾丸支持细胞分离方案;试验发现,牛胎儿睾丸支持细胞体外研究时间应控制在3天～20天内,处于对数生长期的牛胎儿睾丸支持细胞,对牛体外受精卵体外发育有明显的促进作用。     

移植部位对小鼠睾丸移植效果的影响

目的比较不同的移植部位对睾丸移植效果的影响,以探索建立疾病模型小鼠安全保存的新方法。方法按移植部位的不同分为3组:背部皮下组,睾丸白膜内组和肾包膜下组。移植后处死受体鼠回收移植物。测试和分析受体精囊的重量,移植物存活率,回收物增重的倍数和生殖细胞的分化情况。结果不同实验组移植睾丸的生殖细胞分化差异显著。睾丸白膜内组的分化情况最好与假移植对照组相似;背部皮下移植组睾丸的分化率为29.2%;肾包膜下组未见分化。结论睾丸白膜内移植最利于精子的发生;背部皮下移植是睾丸移植的次优选择;肾包膜下睾丸移植不适合用于小鼠雄性生殖器官的安全保存。     

糖尿病治疗新进展——胰岛细胞移植

随着医学科学的发展和生物学技术的进步,胰岛细胞移植已经被认为是治疗1型糖尿病的一种有效方法。技术上首先要解决好移植物的来源、提取和储存。同时,将移植物导入体内的技术也在不断发展,介入放射学技术发挥了非常重要的作用。研究发现．移植后受体的高血糖明显降低,并能在较长时期保持在正常水平。但胰岛细胞移植后,同样面临移植排斥反应,而在应用免疫抑制剂后又可能引起肝小静脉病等不良反应。利用磁共振和光学成像对标记后的胰岛细胞进行显像,对移植后的胰岛细胞在活体内进行追踪．了解其分布和存活,对于长期监测其功能、改进移植技术和免疫调节方法也很重要。目前面临的问题终将逐一得到解决．胰岛细胞移植很有希望成为治愈糖尿病的方法。     

培养大脑皮层神经元的新方法——睾丸支持细胞的应用

In the present study, cerebral cortex neurons were cultured with (named as co-culture group) or without (named as control group) Sertoli cells in vitro, in order to examine the trophic effect of Sertoli cells on the neurons. Our results demonstrated that the growth of the neurons and the viability was enhanced significantly. The increases in the cellular area and number of neurite of the neurons were observed (174.85 +/- 105.18 vs 96.59 +/- 41.63, 2.53 +/- 1.79 vs 1.36 +/- 0.54: P < 0.01). Our study suggests neurons culturing with Sertoli cells is a new and convenient method of obtaining a large number of neurons.     

保护胰岛β细胞的体外研究进展

糖尿病是一种由胰岛素分泌缺陷和（或）胰岛素作用缺陷引起的高血糖症性代谢疾病。自Edmonton临床试验取得成功后,胰岛移植成为一种新型治愈糖尿病的方法。但胰岛β细胞在体外分离过程中极易发生凋亡或死亡,且长期的体外培养或冷冻储存也容易令其胰岛素分泌功能逐渐丧失。因此,有效维持或改善β细胞的成活率及功能对胰岛移植的成功至关重要。对胰岛β细胞的体外保护方法进行阐述,并对其研究前景进行展望。     

镉暴露大鼠睾丸支持细胞金属硫蛋白表达的时相研究

啮齿目动物的睾丸较肝脏对镉毒性更为敏感.为阐明不同组织细胞的镉毒性分子机制,对镉暴露大鼠睾丸支持细胞与肝脏金属硫蛋白基因(MT)的表达及镉蓄积进行了时相研究.成年雄性SD大鼠低剂量镉(4.0 μmol/kg)皮下注射后,立即进行睾丸支持细胞和肝脏组织的分离.采用RT-PCR技术分析mRNA,并用光密度扫描作半定量分析,蛋白质定量用ELISA方法,原子分光光度吸收法测定镉浓度.结果显示：镉暴露1 h后肝脏MT mRNA即有明显的诱导表达,3 h达高峰;支持细胞也有明显的诱导表达, 6 h达高峰.镉暴露后肝脏MT有明显的诱导表达,但睾丸支持细胞不但未见MT增加而且还稍有下降.提示：a.镉对MTmRNA的诱导表达具有时间依赖性和组织特异性.b.镉虽然能诱导睾丸MT的转录,但没有促进其MT的合成,这可能是睾丸对镉毒性与致癌作用较肝脏更敏感的重要原因.     

Synthesis and transport of different sphingomyelin species in rat Sertoli cells

Cellular phospholipids of Sertoli cells from immature rats were labeled with [¹⁴C]-choline. Two sphingomyelin bands (SM1 and SM2) were identified by TLC. The incorporation of [¹⁴C]-choline over a 45 h period of incubation demonstrated that there are differences in labeling kinetics between SM1 and SM2. The subcellular location of SM1 and SM2 was investigated by accessibility to bacterial sphingomyelinase. The results showed the existence of two SM pools in Sertoli cells, but an equal cellular distribution of SM1 and SM2. SM2 is characterized by a relatively high content of unsaturated fatty acids. The inhibition of vesicular flow by monensin determines a decrease of about 60–70% in incorporation into SM1 and SM2, suggesting the existence of at least two sites of sphingomyelin synthesis. Pulse-chase and time-course experiments indicated a phosphatidylcholine SM precursor product relationship and differences in kinetic properties between SM1 and SM2. Resynthesis experiments showed that monensin had only a partial inhibitory effect on SM1 resynthesis, and a second sphingomyelinase treatment demonstrated that the resynthesized fraction reached the outer leaflet of the plasma membrane. The 60–70% inhibition of SM synthesis by monensin showed that the trans-Golgi cisternae and the trans-Golgi network are the most likely sites of bulk SM synthesis, and that about 15% of SM was synthesized in the cis/medial Golgi apparatus. Additionally the results indicated that plasma membrane SM synthase activity could be the site of about 15% of SM synthesis in Sertoli cells.     

Mouse Sertoli cells isolation by lineage tracing and sorting

Sertoli cells play a key role in spermatogenesis by supporting the germ cells throughout differentiation. The isolation of Sertoli cells is essential to study their functions. However, the close contact of Sertoli cells with other testicular cell types and the high proliferation of contaminating cells are obstacles to obtain pure primary cultures. Current rodent Sertoli cell isolation protocols result in enriched, rather than pure Sertoli cells. Therefore, novel approaches are necessary to improve the purity of Sertoli cell primary cultures. The goal of this study is to obtain pure mouse Sertoli cells using lineage tracing and fluorescence‐activated cell sorting (FACS). We bred the Amh‐Cre mouse line with tdTomato line to generate mice constitutively expressing red fluorescence specifically in Sertoli cells. Primary cultures of Sertoli cells isolated from prepubertal mice showed that 79% of cells expressed tdTomato, as evaluated by fluorescence microscopy and flow cytometry; however, nearly all adherent cells were positive for vimentin. Most of the tomato‐negative cells expressed α‐smooth muscle actin (α‐SMA), a peritubular myoid cell marker, but double‐negative populations were also present. These findings suggest that vimentin lacks Sertoli cell‐specificity and that α‐SMA is not adequate to identify all of the contaminating cells. Upon FACS sorting; however, virtually 100% of the cells were tdTomato positive, expressed vimentin, but not α‐SMA. Prepubertal mice yielded a higher number of Sertoli cells compared to adults, but both could be adequately sorted. In conclusion, our study shows that lineage tracing and sorting is an efficient strategy for acquiring pure populations of murine Sertoli cells.     

Fine structure of Sertoli cells in three marine snails with a discussion on the functional morphology of Sertoli cells in general

Summary The fine structure of Sertoli cells in three marine prosobranch molluscs has been studied with light- and electron microscopy. Sertoli cells of prosobranchs are modified columnar epithelial cells that maintain continuous contact with the basal lamina and extend from it to the lumen of a testicular tubule. Spermatogenesis takes place between adjacent Sertoli cells, but a continuous layer of cytoplasm separates the spermatogonia from the basal lamina, thus restricting the basal compartment to spermatogonium mother cells. Substances traversing the basal lamina from the interstitial space must pass either through or between the Sertoli cells. However, between the cells, a permeability barrier composed of septate and desmosome-like junctions blocks the passage of substances, such as the tracer lanthanum nitrate. The basally-located nucleus is irregularly shaped with fine granular euchromatin and some peripheral heterochromatin; satellite karyosomes border the nucleolus. There is an extensive intracellular digestive system that is used effectively to phagocytize waste sperm and residual cytoplasm. Cytoplasmic processes of Sertoli cells penetrate throughout the germinal epithelium. In some prosobranchs that exhibit sperm polymorphism these processes must coordinate to bring together a clone of eupyrene sperm and a carrier sperm at a particular time in development. The only cytoskeletal elements available within the processes to generate such movements are microtubules.We propose that the term nurse cell, which has been used in the past to describe at least three different cell types, including Sertoli cells and apyrene sperm, be restricted to abortive oogonia that contribute to development of an oocyte.This paper was cited in a previous publication (Buckland-Nicks et al. 1982) under the title: A comparative investigation into the relationship between Sertoli cells, eupyrene and apyrene sperm in the testis of two marine snails     

以支持细胞为饲养层培养小鼠精原干细胞

为探索精原干细胞(Spermatogonialstemcells,SSCs)体外自增殖的条件以及SSCs体外快速扩增的方法,以6-8日龄昆明乳鼠为材料,分离小鼠睾丸细胞,采用Percoll梯度离心法富集SSCs;以经丝裂霉素C处理的Sertoli细胞作饲养层,以DMEM为基本培养基,加入5%胎牛血清和103u/ml的白血病抑制因子(Leukemiainhibitoryfactor,LIF),体外培养SSCs;运用免疫荧光技术,以SSCs特异性表面分子Thy1为标志,对原代培养20d和传代培养14d的细胞进行鉴定。该培养体系下,SSCs贴壁时间为6h-9h,48h后可见细胞分裂,迅速增殖出现在接种12d以后。接种后第20d形成数十至上百个细胞的细胞团,细胞总数比接种时增加了45-245倍,100倍显微镜下观察可见,单位视野内细胞团数为26±4个。传代后细胞增殖较快。原代培养20d和传代培养14d的细胞均为Thy1阳性;而传代20d后,细胞周缘不整,有伪足出现,呈现出死亡迹象。该培养条比较适合SSCs短期快速增殖。     

Alpha-1-antitrypsin immunoreactivity in islet cells of adult human pancreas

alpha-1-antitrypsin immunoreactivity was demonstrated by immunofluorescence technique in the peripheral islet cells of all ten normal adult human pancreata examined; normal adult human liver was negative. The specificity of the reactions was confirmed by applying various control tests including absorption of the specific antisera with purified alpha-1-antitrypsin, inhibition and blocking tests and by ensuring the monospecificity of the antisera used. The findings suggest that the pancreatic islet may be an additional source of alpha-1-antitrypsin.     

Pioglitazone increases the glycolytic efficiency of human Sertoli cells with possible implications for spermatogenesis

Pioglitazone is a synthetic agonist for the nuclear receptor peroxisome proliferator-activated receptor γ used to treat type 2 diabetes mellitus. Recently we reported that antidiabetic drugs regulate the nutritional support of spermatogenesis by Sertoli cells. Herein, we investigate the effects of pioglitazone on human Sertoli cells metabolism. Human Sertoli cells were cultured in the presence of pioglitazone (1, 10, 100 μM). Protein levels of phosphofructokinase 1, lactate dehydrogenase, hexokinase, glucose transporters (GLUT1, GLUT2, GLUT3), monocarboxylate transporter 4 and oxidative phosphorylation complexes were determined by Western blot. Lactate dehydrogenase and alanine aminotransferase activity were assessed and metabolite production and consumption determined by proton nuclear magnetic resonance. Mitochondrial membrane potential was also determined. Glucose consumption more than doubled in human Sertoli cells stimulated with pioglitazone 100 μM. Mitochondrial complex II protein levels increased 50% with exposure to pioglitazone (100 μM) in human Sertoli cells, though mitochondrial membrane potential was decreased by 32%. The pharmacological concentration of pioglitazone (10 μM) almost doubled lactate production and established crucial correlations among key intervenient of glycolysis. Moreover, in the same concentration, alanine aminotransferase decreased more than 80%. Our results suggest that pioglitazone (10 μM) increases the efficiency of the glycolytic flux and lactate production by human Sertoli cells, which is essential to sustain and preserve the spermatogenic event. Thus, pioglitazone may improve male fertility and thus, be considered a suitable antidiabetic drug for men in reproductive age.     

Testicular Sertoli cells influence the proliferation and immunogenicity of co-cultured endothelial cells

The major problem of the application of endothelial cells (ECs) in transplantation is the lack of proliferation and their immunogenicity. In this study, we co-cultured ECs with Sertoli cells to monitor whether Sertoli cells can influence the proliferation and immunogenicity of co-cultured ECs. Sertoli cells were isolated from adult testicular tissue. ECs were divided into the control group and the experimental group, which included three sub-groups co-cultured with 1 × 10³, 1 × 10⁴ or 1 × 10⁵ cell/ml of Sertoli cells. The growth and proliferation of ECs were observed microscopically, and the expression of vascular endothelial growth factor (VEGF) receptor-2 (KDR) was examined by Western blotting. In another experiment, ECs were divided into the control group, the single culture group and the co-culture group with the optimal concentration of Sertoli cells. After INF-γ and TNF-α were added to the culture medium, MHC II antigen expression was detected by immunofluorescence staining and western blotting; interleukin (IL)-6, IL-8 and soluble intercellular adhesion molecule (sICAM) were measured in the culture medium by ELISA. We demonstrated that 1 × 10⁴ cell/ml Sertoli cells promoted the proliferation of co-cultured ECs more dramatically than that in other groups (P < 0.05). Western blotting showed that 1 × 10⁴ cell/ml of the Sertoli cells was most effective in the up-regulation of KDR expression in the co-cultured ECs (P < 0.05). Sertoli cells can effectively suppress INF-γ-induced MHC II antigen expression in co-cultured ECs compared with single culture group (P < 0.05). TNF-α induced the expression of IL-6, IL-8 and sICAM in ECs. When co-cultured with Sertoli cells, their expressions were significantly lower than in the EC single culture group (P < 0.05). ECs co-cultured with Sertoli cells also did not significantly increase the stimulation index of spleen lymphocytes compared to the single culture group (P < 0.05). Our results suggested that co-culturing with Sertoli cells can significantly promote the proliferation of ECs, accelerate post-transplant angiogenesis, while reduce EC immunogenicity and stimulus to lymphocytes.     

Retinol and retinoic acid increase MMP-2 activity by different pathways in cultured Sertoli cells

Diseases such as atherosclerosis, arthritis and cancer have been related with imbalance in ROS production and failures in regulation of the MMPs. Authors suggested a relationship between MPP activity and ROS. Our research group has demonstrated that retinol 7µM induced changes in Sertoli cell metabolism linking retinol treatment and oxidative stress. We verified MMP activity in Sertoli cells treated with vitamin A using gelatin zymography. We found that retinol (7µM) and retinoic acid (1nM) induced MMP-2 activity in Sertoli cells. Antioxidants reversed retinol-induced but not retinoic acid-induced MMP-2 activity. Moreover, retinol but not retinoic acid increased ROS production quantified by DCFH-DA oxidation. We found that retinol and retinoic acid induced ERK1/2 phosphorylation, but only retinol-increased MMP-2 activity was inhibited by UO126, an ERK1/2 phosphorylation inhibitor. Our findings suggested that retinol-induced MMP-2 activity, but not retinoic acid-induced MMP-2 activity, was related to ERK1/2 phosphorylation and ROS production.     

Sertoli and Leydig cell numbers and gonadotropin receptors in rat testis from birth to puberty

Summary In testes of rats from 2 to 60 days of age, we examined the number of Sertoli cells (SC) and Leydig cells (LC) as well as the binding of radioiodinated gonadotropins to frozen sections and homogenates. The number of SC per testis increased only during the first 2 postnatal weeks, whereas that of LC was stable up to days 7–10 and increased thereafter. The uptake of ¹²⁵I-labelled human follicle-stimulating hormone (¹²⁵I-FSH) to frozen sections was confined to sex cords or seminiferous tubules, while that of ¹²⁵I-labelled human choriogonadotropin (¹²⁵I-hCG) matched the distribution of LC in the interstitium. High affinity receptors for FSH and hCG were found in homogenates at all stages studied. The number of FSH receptors per testis increased steadily, whereas that of hCG receptors was low until days 7–10 and rose afterwards. Thus, SC in rat testis appear to proliferate in the presence of fetal LC during the first 2 postnatal weeks and to differentiate concomitantly with the emergence of the adult LC generation after day 10. The complement of FSH receptors in SC remains constant as they proliferate and increases after day 21 as they differentiate. The hCG receptor number is relatively fixed in each LC generation, being higher in adult compared to fetal LC.     

Retinol and retinoic acid increase MMP-2 activity by different pathways in cultured Sertoli cells

Diseases such as atherosclerosis, arthritis and cancer have been related with imbalance in ROS production and failures in regulation of the MMPs. Authors suggested a relationship between MPP activity and ROS. Our research group has demonstrated that retinol 7µM induced changes in Sertoli cell metabolism linking retinol treatment and oxidative stress. We verified MMP activity in Sertoli cells treated with vitamin A using gelatin zymography. We found that retinol (7µM) and retinoic acid (1nM) induced MMP-2 activity in Sertoli cells. Antioxidants reversed retinol-induced but not retinoic acid-induced MMP-2 activity. Moreover, retinol but not retinoic acid increased ROS production quantified by DCFH-DA oxidation. We found that retinol and retinoic acid induced ERK1/2 phosphorylation, but only retinol-increased MMP-2 activity was inhibited by UO126, an ERK1/2 phosphorylation inhibitor. Our findings suggested that retinol-induced MMP-2 activity, but not retinoic acid-induced MMP-2 activity, was related to ERK1/2 phosphorylation and ROS production.