人体皮肤成纤维细胞的快速分离及多向分化能力鉴定

目的建立快速分离人皮肤成纤维细胞的方法,并探讨成纤维细胞在成脂、成骨、成软骨和成神经的多向分化潜能。 方法利用组织块培养法分离人体皮肤成纤维细胞,通过形态学观察、流式分析、Vimentin蛋白染色鉴定成纤维细胞;再利用生长曲线、核型分析、线粒体染色分析不同传代细胞的增殖速度,线粒体及染色体形态的改变;最后进行成纤维细胞成脂、成骨、成软骨和成神经的诱导分化实验,鉴定其多向分化潜能。两代细胞增殖速度及线料体相对量的比较采用t检验统计分析。 结果分离的皮肤成纤维细胞呈典型梭状及多角形;高表达细胞表面标记物CD90 （NCF1,NCF2占比分别为99.9%,98.7%）和CD73 （NCF1,NCF2占比分别为98.2%,85.6%）,但极少表达造血干细胞标记物CD34 （NCF1,NCF2占比分别为1.8%,2.6%）;细胞Vimentin蛋白表达呈阳性,阳性率为100%;对细胞生长曲线进行分析,表明分离后不同代次细胞增殖差异无统计学意义（t?= 1.586,P?= 0.1567）;线粒体相对含量统计分析,同一株细胞系第5代（相对荧光强度值：6876±577.8）与第10代（相对荧光强度值：7371±471.9）之间的差异无统计学意义（t?= 0.664,P?= 0.543）;核型分析分别显示传代后保持染色体数目为正常46条且形态无明显异常;经诱导后成纤维细胞可向成脂、成骨、成软骨和类神经分化。 结论利用组织块培养法分离出的人体皮肤成纤维细胞状态稳定,增殖能力强,具有成脂、成骨、成软骨和成神经多向分化诱导潜能,为细胞移植修复骨损伤、软骨损伤和神经损伤性疾病的临床研究提供细胞来源及实验依据。     

东方田鼠皮肤成纤维细胞的分离培养及生物学特性

目的探索和建立东方田鼠皮肤成纤维细胞体外分离、培养的技术方法并观察其生物学特性。方法采用含10%小牛血清的Dulbecco改良Eagle培养液(DMEM)和1640两种培养体系,运用组织块贴壁法和胰酶消化法,分别对出生后1、3 d和5 d的东方田鼠乳鼠皮肤成纤维细胞进行原代分离、培养。苏木素-伊红染色及倒置相差显微镜下观察成纤维细胞形态和生长特性。结果 0.25%胰酶消化分离出生后1 d和3 d东方田鼠乳鼠皮肤较出生后5 d组织可获得较多数量细胞,成纤维细胞在体外快速贴壁生长,一般6～7 d长满培养瓶,细胞纯度高,HE染色细胞呈长梭形,胞核明显;DMEM和1640两种培养液均可用于东方田鼠皮肤成纤维细胞的培养,但细胞传代后生长趋缓,只可传代2～3次。本实验运用组织块贴壁法未能培养出皮肤成纤维细胞。结论确定了有效分离东方田鼠皮肤成纤维细胞的日龄和方法,为进一步深入研究提供了技术方法和操作依据。     

成年大鼠嗅鞘细胞与嗅觉神经成纤维细胞的原代培养及鉴定

目的 建立一种原代提取嗅鞘细胞与嗅觉神经成纤维细胞混合培养的方法.方法 自2.5月龄SD大鼠嗅球最外两层分离嗅鞘细胞和嗅觉神经成纤维细胞进行混合培养,并不进行纯化,分别于7 d、10 d、14 d行免疫细胞化学鉴定,并计算各个时间点嗅鞘细胞的纯度.结果 体外培养的嗅鞘细胞主要呈两极或多极状,而嗅觉神经成纤维细胞则成扁平的像成纤维细胞的形态,免疫细胞化学结果显示嗅鞘细胞呈p75 NGFR阳性,嗅觉神经成纤维细胞呈fibronectin阳性,两种细胞都呈vimentin阳性,在7 d、10 d、14 d各个时间点嗅鞘细胞分别占混合培养的34.1%、25.6%、8.6%.结论 从成年大鼠嗅球最外两层分离的培养中主要包含嗅鞘细胞和嗅觉神经成纤维细胞,嗅鞘细胞在混合培养中所占的比例随培养时间的延长而逐渐降低.     

人正常食管鳞状上皮不同原代培养方法的比较

该研究通过比较人正常食管鳞状上皮不同的原代培养方法,以期为不同的实验目的提供不同的培养方法。实验用到的正常食管粘膜上皮来源于食管癌患者手术切除的标本,采用组织块法和酶消化法,分别用DMEM/F12混合培养基和K-SFM无血清培养基进行培养。通过直接观察、细胞形态学观察和免疫细胞化学方法观察细胞的生长情况、细胞形态学特征及鉴定所得到的细胞,比较不同方法与不同培养基组合中原代培养细胞的生长状况。用组织块法,在DMEM/F12混合培养基中人正常食管上皮细胞生长较好,细胞融合较快,成纤维细胞污染较少,15～17天上皮细胞铺满瓶底的70%～80%,获得的细胞数量大,但细胞传代后成纤维细胞污染严重。用酶消化法,在K-SFM无血清培养基中人正常食管上皮细胞生长好,细胞融合快,成纤维细胞污染基本消除,细胞纯度高,10～12天细胞便可以铺满瓶底的70%～80%,这种方法培养的细胞可以冻存、复苏和传代。其余各种培养方法所得细胞无论在生长状态、培养周期、成纤维细胞污染和传代方面均较前两种方法差。以上各种方法培养的细胞经免疫细胞化学染色鉴定证实细胞呈广谱细胞角蛋白阳性,确定是食管上皮来源的细胞。酶消化法加K-SFM无血清培养基是本实...     

水牛皮肤成纤维细胞的分离与体外培养

探讨水牛成纤维细胞的分离与传代培养方法。组织块培养法培养的成纤维细胞原代生长较慢,需12天左右方可汇合形成单层,而酶消化法培养的成纤维细胞原代生长相对生长快,仅需8天便可汇合形成单层。两种方法传代细胞的生长速度相似,仅需4-5天就可汇合形成单层。通过体细胞的核型分析发现,成纤维细胞在传代培养过程中的核型变化不大,66．67％～81．67％的细胞具有正常的二倍体核型,各代之间无显著差异。结果表明,水牛成纤维细胞均能稳定地进行传代培养。     

自发性可移植性615小鼠肺癌和肝癌组织神经节苷脂高效薄层层析图谱的分析

本文研究了615近交系小鼠的自发性可移植性肺癌(P_(615))和肝癌(H_(615))组织中神经节苷脂结合唾液酸含量和神经节苷脂图谱。P_(615)和H_(615)癌组织中GLS结合唾液酸含量均比正常对照为高,分别为对照组织的2.9倍和1.9倍。615小鼠的正常肺组织和肝组织的GLS主要成分均为GM_3。在P_(615)和H_(615)癌组织中GM_3含量均明显减少。肺癌组织中GM_2大量增加,肝癌组织中不仅GM_2明显增加,GM_1和GD_(18)也明显增加。P_(615)和H_(615)这两种分化程度较高、恶性程度较低的癌组织GD_3的百分含量比正常对照组织略有降低。本文结果提示,自发性可移植性P_(615)和H_(615)肿瘤组织中不仅神经节苷脂含量(以唾液酸量计)升高,而且GLS的组分也发生改变。GM_3含量减少和GM_2含量增高可能与肿瘤的恶性生长和分化程度有关。     

猪耳皮肤成纤维细胞的培养

本研究以猪耳皮组织为材料,采用胰蛋白酶冷热处理结合法成功地分离和培养了猪耳皮肤成纤维细胞。此方法的细胞存活率相对于胰蛋白酶热处理法较高。传代细胞与原代细胞的形态和生长速度均相似。传代细胞未检测到凋亡现象。细胞已传至15代以上,染色体倍性正常,说明我们所建立的胰蛋白酶冷热处理结合法可以快速有效的分离和培养猪耳皮肤成纤维细胞,并且能稳定的进行传代培养。     

高效薄层层析-病毒覆盖结合法比较细胞表面神经节苷脂与不同动物源性新城疫病毒结合特性

【目的】神经节苷脂是新城疫病毒入侵宿主细胞的受体,但不同动物源性的新城疫病毒利用受体的特性是否存在差异尚不明确。以鹅源新城疫病毒NA-1株和鸡源新城疫病毒F48E9株为研究对象,比较两株病毒受体结合特性的差异。【方法】提取鸡胚和鹅胚成纤维细胞新城疫病毒受体成分——神经节苷脂,用高效薄层层析法比较两种细胞所含神经节苷脂的类型和含量;通过高效薄层层析-病毒覆盖结合法比较两种病毒与不同细胞神经节苷脂的结合特性,最后通过病毒红细胞吸附抑制试验进一步验证神经节苷脂与病毒之间的相互作用关系。【结果】鸡胚和鹅胚成纤维细胞所含的神经节苷脂成分存在明显差异;高效薄层层析-病毒覆盖结合实验结果显示NA-1和F48E9与神经节苷脂的结合模式不同,NA-1主要与神经节苷脂GD1a结合,即包含双SAα2,3Gal末端的神经节苷脂,而F48E9可与更多类型的神经节苷脂结合,从单唾液酸到三唾液酸形式的神经节苷脂如GM1、GD1a、GD1b、GT1b等。【结论】鹅源新城疫病毒NA-1株和鸡源新城疫病毒F48E9株在入侵靶细胞时优先选择利用的受体不同。     

ICR胎鼠成纤维细胞培养方法的优化

目的确定胎鼠成纤维细胞（mouse embryonic fibroblasts,MEF）最优制备方法,为MEF的制备节省时间与原材料。方法取胎鼠组织,采用组织块培养法、胰酶消化培养法、胰酶消后组织块培养法进行分离培养MEF,比较观察MEF纯度、生长速度、细胞形态等指标,筛选最节省时间与原料的一种培养方法。结果组织块培养法所得MEF生长速度慢,细胞体积小,杂细胞少,纯化所需传代次数少。胰酶消化培养法的MEF生长速度快,体积较大,杂细胞数量多,纯化所需传代次数较多。胰酶消化后组织块培养法的消化后组织块的成纤维细胞生长速度介于前两种方法之间,细胞体积和形态与组织块法培养结果相似,杂细胞数量较少,纯化所需传代次数少。结论胰酶消化结合组织块培养法能最大限度的利用材料,在短时间内可制备大量MEF,满足核移植试验与作为饲养层细胞的需求。因此,胰酶消化结合组织块培养法是MEF最优培养方法。     

肠道菌的细胞受体——神经节苷脂

<正>神经节苷脂是天然的有机结合物,它是一种复杂的脂质(甘氨酸神经氨基醇脂)并含有残余的唾液酸,是大多数有生物活性分子的全适受体。它们是细胞和哺乳动物的组织成分,但以脑组织较为丰富,因此,通常以此作为获得神经节苷脂的来源,其亲水部分在细胞膜外面,主要成分有:葡萄糖、半乳糖、N—乙醛基半乳糖、N—乙酰基神经氨基酸,而疏水部分包括(神经)鞘氨醇和     

Measurement of DNA polymerase beta in skin fibroblast cell lines from patients with ataxia telangiectasia

DNA polymerase beta levels were measured in 4 cell lines of normal human skin fibroblasts and in 5 cell lines of skin fibroblasts from patients with ataxia telangiectasia, an autosomal recessive disease exhibiting marked X-ray sensitivity. The enzyme specific activities for the normal lines were similar and the mean value was 2-fold lower than the mean value for the ataxia lines. With both kinds of cells, the enzyme level did not change as the cultures progressed from logarithmic to stationary phase of growth. Thus, this putative DNA repair enzyme appears to be 'constitutive' in human skin fibroblast lines, and a modest elevation of beta-polymerase activity is associated with ataxia telangiectasia. These results are discussed in the context to current views about DNA-repair enzymes in X-ray-sensitive cultured mammalian cells.     

Tay-Sachs and Sandhoff''s disease: Intergenic complementation after somatic cell hybridization

Cultivated skin fibroblasts from patients with Tay-Sachs and Sandhoff's disease were fused and the isoenzymes of N-acetyl-β- -hexosaminidase were investigated after 2 and 7 days of subsequent cultivation. Enzyme analyses after heat inactivation showed a clear increase in the thermolabile component of hexosaminidase when compared with assays on fusion of each of the parental cell strains. Electrophoretic studies revealed that in cell homogenates prepared at various time intervals after cell fusion of Tay-Sachs with Sandhoff's fibroblasts, all three hexosaminidase isoenzymes were present, including hexosaminidase A which lacks in both parental cell strains. These results show that genetic complementation has occurred, which indicates that two different gene mutations are involved in these variants of GM2-gangliosidosis. The relevance of the data obtained for the elucidation of the molecular properties of the (iso)enzymes involved is discussed.     

Mitogenic effects of bacterial neuroaminidase and lactosylceramide on human cultured fibroblasts.

Exogenously added bacterial neuraminidase and lactosylceramide both stimulated the growth of cultured human skin fibroblasts. Neuraminidase (100 units/ml) increased DNA synthesis 1.9-fold and cell density 1.4-fold after 24 and 48 h, respectively, in culture. Treated fibroblasts contained less ganglioside NeuAc alpha 2-3Gal beta 1-4GlcCer (GM3), presumably due to neuraminidase-catalyzed hydrolysis to lactosylceramide. Addition of lactosylceramide (100 microM) to the fibroblast culture medium also increased DNA synthesis threefold within 24 h and cell density twofold after 48 h. These findings are compatible with a mechanism by which the proliferation of human fibroblasts is regulated by the relative levels of GM3 and lactosylceramide in the plasma membrane.     

Phospholipids and glycosphingolipids in cultured skin fibroblasts from healthy donors and patients with systemic scleroderma

A comparative study of phospho- and glycosphingolipids of cultured skin fibroblast from healthy donors and from patients with systemic sclerodermia (SSD) was carried out. It was shown that the total phospholipid content in SSD fibroblasts is elevated. No significant changes in the concentration of neutral glycosphingolipids were observed. The ganglioside composition of SSD cell cultures differs significantly from that of healthy donor cells. The concentration of the gangliosides, GM3 and GM1, is decreased; no ganglioside GD1a was found in SSD fibroblasts. The data obtained are suggestive of changes in the properties of fibroblast surface which can be manifested both in the impaired reception of matrix proteins and in the impairment of basic properties of the membrane. These changes are well correlated with the results of previous studies on the AMP cyclase system.     

Utilization of electron microscopy in the prenatal diagnosis of genetic disease.

The use of electron microscopy as a further method of diagnosis of disease in cultured skin fibroblasts and cultured amniotic fluid fibroblasts is presented. It was demonstrated that Tay-Sachs disease, Fabry's disease, and metachromatic leukodystrophy had distinctive abnormalities in both cultured skin fibroblasts and cultured amniotic fluid fibroblasts. It was shown that control of culturing conditions made it possible to distinguish normal cell lines from certain cell lines carrying known genetic diseases.     

Nuclear complementation restores mtDNA levels in cultured cells from a patient with mtDNA depletion.

We have studied cultured skin fibroblasts from a patient with a fatal mitochondrial disease manifesting soon after birth. These fibroblasts were found to grow only in the presence of pyruvate and uridine, a characteristic of cells lacking mtDNA (rho0 cells). Southern blot and PCR analyses confirmed that the patient's fibroblasts contained less than 2% of control levels of mtDNA. Biochemical analyses indicated that the activities of all the respiratory-chain enzymes were severely decreased in mitochondria isolated from these fibroblasts. In order to elucidate the underlying molecular defect, cell fusions were performed between enucleated fibroblasts from this patient and a human-derived rho0 cell line (rho0 A549.B2). The resulting cybrids were plated in medium lacking pyruvate and uridine, to select for the restoration of respiratory-chain function. Complementation was observed between the nuclear genome of the rho0 A549.B2 cells and the mtDNA of the patient's cells, restoring mtDNA levels and respiratory-chain function in the cybrid cells. These results indicate that mtDNA depletion in our patient is under the control of the nuclear genome.     

Studies on complementation of beta hexosaminidase deficiency in human GM2 gangliosidosis.

Complementation of beta hexosaminidase A (hex A) deficiency was obtained by Sendai virus-mediated somatic cell hybridization of cultured skin fibroblasts from two unrelated patients with Tay-Sachs disease (TSD) and one patient with Sandhoff-Jatzkewitz disease (SJD). The newly formed hex A was identified by its electrophoretic mobility in three different systems, heat lability, and reactivity with an antiserum against the unique antigenic determinant, alpha of hex A. The percentage of heterokaryons obtained by virus treatment of TSD and SJD fibroblast mixtures showed good correlation with the observed percentage of hex A activity. It is concluded that, in these two forms of GM2 gangliosidosis, beta hexosaminidase deficiency results from two different mutations. All of the current models of beta hexosaminidase structure are compatible with the observed complementation. No complementation was detected in 13 Sendai virus-induced fusions of cultured skin fibroblasts from seven unrelated patients with SJD. The enzyme deficiency in these patients may be due to very similar allelic mutations, not capable of undergoing complementation; or to different structural mutations, all coding for unstable beta hexosaminidase molecules.     

Incorporation and degradation of GM1 ganglioside and asialoGM1 ganglioside in cultured fibroblasts from normal individuals and patients with beta-galactosidase deficiency

The uptake and degradation of GM1 ganglioside (GM1) and asialoGM1 ganglioside (GA1) were studied in cultured fibroblasts from normal individuals and patients with beta-galactosidase deficiency, using the lipid-loading test. The glycolipids were incorporated from the media into the fibroblasts and the terminal galactose was hydrolyzed in normal cells. The hydrolysis rates of GA1 were 80-86% of normal on the 3rd day after loading, while GM1 was hydrolyzed slowly; 35-54% on the 14th day. In infantile GM1 gangliosidosis and I-cell disease, little GM1 and GA1 was hydrolyzed on any day of culture, while fibroblasts from patients with adult GM1 gangliosidosis, Morquio disease type B and galactosialidosis hydrolyzed the lipids at nearly normal rates. The intracellular accumulation of the glycolipids, on the basis of protein content, was abnormally high in the case of infantile GM1 gangliosidosis and I-cell disease, but normal in the other disorders examined. These observations indicate that the in situ metabolism of GM1 and GA1 is probably normal in fibroblasts from patients with adult GM1 gangliosidosis, Morquio disease type B and galactosialidosis, although in vitro beta-galactosidase activities in these disorders are very low. The results are compatible with findings that GM1 and GA1 do not accumulate in the somatic organs of patients with adult GM1 gangliosidosis and galactosialidosis. In I-cell disease, however, the results of the loading test did not agree with the finding that there is little accumulation of glycolipids in postmortem tissues.     

Effect of lectins on endocytosis and secretion of lysosomal enzymes by cultured fibroblasts.

1. Pretreatment of cultured human skin fibroblasts with convanavalin A and wheat germ agglutinin inhibited endocytosis of alpha-N-acetylglucosaminidase and increased extracellular accumulation of beta-N-acetylglucosaminidase. 2. These effects were dose-dependent, reversible and could be prevented by haptenic carbohydrates, such as methyl alpha-D-mannoside or N-acetylglucosamine. 3. Pretreatment of fibroblasts with di- and monovalent succinylated concanavalin A inhibited alpha-N-acetylglucosaminidase endocytosis, but had no effect on extracellular beta-N-acetylglucosaminidase accumulation. 4. Concanavalin A-alpha-N-acetylglucosaminidase complexes become internalized via the recognition of the lectin. Complex formation prevents recognition of the phosphorylated carbohydrate on lysosomal enzymes that interacts with cell surface receptors specific for lysosomal enzymes. The inhibitory effect of all lectins tested on lysosomal enzyme endocytosis suggests that the cell surface receptors for lysosomal enzymes interact either directly with lectins or are closely linked to lectin receptors. The effect of polyvalent lectins on extracellular lysosomal enzyme accumulation is ascribed to their alteration of membrane fluidity.     

Heterogeneity for adenosine deaminase deficiency: Expression of the enzyme in cultured skin fibroblasts and amniotic fluid cells.

Adenosine deaminase (ADA) could be quantitated and the isozyme pattern characterized in cultured amniotic fluid cells. In 20 amniotic fluid cell cultures the mean specific activity was 14.3 U/g protein +/- 6.7 (SD) and compared favorably with values of 14.6 U/g protein +/- 6.8 (SD) observed in 26 cultures of skin fibroblasts. In cultures of skin fibroblasts established from two obligate heterozygotes for ADA deficiency, the specific activity of ADA was 7.0 and 7.7 U/g protein. The ADA isozyme pattern that existed in cultures of amniotic fluid cells was the same as that observed in cultured skin fibroblasts. This identification of the same apparent enzyme may permit the prenatal diagnosis of that form of combined immunodeficiency disease caused by ADA deficiency. Residual enzyme activity of less than 1% and 10% of the mean of normal fibroblasts could be measured in cultured fibroblasts from two unrelated children with ADA deficiency and combined immunodeficiency disease. The tissue-specific enzyme from cultured skin fibroblasts from the child with 10% residual activity had a faster electrophoretic mobility and greater heat stability than normal ADA. This enzymatic evidence indicates that at least two mutant alleles exist at the locus for ADA which predispose to combined immunodeficiency disease when present in the homozygous state.