N-乙酰半胱氨酸对大鼠心脏成纤维细胞增殖和胶原合成的影响

目的:通过观察N-乙酰半胱氨酸(NAC)对大鼠心脏成纤维细胞(CFs)增殖和胶原合成的影响,探讨NAC对心脏重构的作用。方法:以培养的新生SD大鼠CFs为实验对象,给予不同浓度的NAC进行干预,48小时后用MTT比色法检测CFs增殖水平,用3H脯氨酸掺入法测定总胶原合成。结果:与对照组相比,不同浓度NAC作用下的CFs增殖水平和3H脯氨酸掺入量均比对照组低,且具有浓度依赖性(p<0.05)。结论:NAC能够抑制SD大鼠CFs增殖,并降低其胶原合成,因此NAC对心脏的病理性重构可能具有保护作用。     

N-乙酰半胱氨酸对大鼠心脏成纤维细胞增殖和胶原合成的影响

目的：通过观察N-乙酰半胱氨酸（NAC）对大鼠心脏成纤维细胞（CFs）增殖和胶原合成的影响,探讨NAC对心脏重构的作用。方法：以培养的新生SD大鼠CFs为实验对象,给予不同浓度的NAC进行干预,48小时后用MTT比色法检测CFs增殖水平,用3H脯氨酸掺入法测定总胶原合成。结果：与对照组相比,不同浓度NAC作用下的CFs增殖水平和3H脯氨酸掺入量均比对照组低,且具有浓度依赖性（p〈0.05）。结论：NAC能够抑制SD大鼠CFs增殖,并降低其胶原合成,因此NAC对心脏的病理性重构可能具有保护作用。     

以人皮肤成纤维细胞作为饲养层细胞培养人胚胎干细胞

目的：比较人皮肤成纤维细胞（humandermalfibroblasts,HDFs）与小鼠胚胎成纤维细胞（Mouseembryonicfibroblasts,MEFs）的增殖能力及研究人皮肤成纤维细胞作为饲养层支持人胚胎干细胞（humanembryonicstemcells,hESCs）未分化生长的能力。方法：利用组织贴壁法从人皮肤中分离出HDFs,通过细胞形态的观察和生长曲线的绘制比较HDFs与MEFs的体外增殖能力。将HDFs作为饲养层细胞与hESCs共培养,传代12代后,检测hESCs碱性磷酸酶（AKP）、表面特异性标志及胚胎干细胞特异性转录因子。结果：HDFs可连续传代培养15代以上,10代以下的HDFs增殖迅速,而MEFs自第4代起,增殖能力就明显下降;hESCs在HDFs饲养层上可传代培养12代以上,克隆边界清晰,细胞排列紧密,碱性磷酸酶、表面标志物检测均呈阳性,表达了hESCs特异性转录因子。结论：HDFs比MEFs具有更强的增殖能力;HDFs可作为培养hEscs的饲养层细胞。     

拟南芥甘露糖苷酶Ⅰ和人 N-乙酰葡萄糖胺转移酶Ⅰ的原核表达及其多克隆抗体制备

目的：在大肠杆菌中分别重组表达拟南芥甘露糖苷酶Ⅰ（ATMDSI）和人N-乙酰葡萄糖胺转移酶I（HsGnTI）,制备其多克隆抗体,为基因表达鉴定提供检测抗体。方法：用PCR方法克隆ATMDSI、HsGnTI基因片段,连接至pBV220表达载体后转化大肠杆菌DH5α,获得表达菌株,通过42℃升温诱导表达,制备纯化ATMDSI和HsGnTI;纯化的蛋白以80μs／ks的剂量免疫大耳白兔,经3次免疫后,采集血清制各其相应的多克隆抗体;采用Western印迹检测多克隆抗体的特异性。结果：获得ATMDSI和HsGnTI基因片段,并构建了其相应的原核表达载体pBV220-ATMDSI、pBV220-HsGnTI,在大肠杆菌中表达了重组ATMDSI和HsGnTI,SDS-PAGE分析显示其相对分子质量分别为45．3×10^3和46．9×10^3,与理论值一致;用纯化的蛋白免疫大耳白兔后制备了抗ATMDSI、HsGnTI多克隆抗体,Western印迹结果证明该抗体具有较高的特异性。结论：获得了特异性较高的抗ATMDSI、HsGnTI多克隆抗体血清,为甘露糖苷酶Ⅰ和N-乙酰葡萄糖胺转移酶Ⅰ的研究提供了检测抗体。     

逆转录病毒介导人VEGF在兔皮肤成纤维细胞中的表达

A replication-deficient recombinant retrovirus containing the cDNA coding for human vascular endothelial growth factor (VEGF) was generated, and then infected rabbit primary skin fibroblasts. After selection with G418, the transduced colonies have the ability of producing VEGF. The integration and expression of VEGF in transduced cells were confirmed by Southern blot, PCR, Northern blot and RT-PCR assay. The VEGF secreted by transduced cells has strong bioactivity when assayed by endothelial proliferation and Miles vascular permeability assay. Thus, this study pave the way for future study of biological and physiological effect of VEGF in vivo.     

皮肤成纤维细胞永生化的研究进展

正常体细胞的生命周期都是有限的 ,经过一定数目的分裂后 ,会进入增殖抑制状态。永生化细胞是近年来生物科学探索较多的领域之一。因为它不仅能为细胞生物学的研究提供性状稳定的研究对象 ,还为人类实现器官再生开辟了新方向。所以皮肤成纤维细胞的永生化对于皮肤疾病以及皮肤组织工程的研究都具有非常深远的意义。就皮肤成纤维细胞的永生化的研究作一阐述 ,并讨论其应用前景和可能面临的问题     

皮肤成纤维细胞肌内注射表达外源基因的可行性

将分别带有报告基因lacZ和人凝血因子ⅨcDNA的兔原代皮肤成纤维细胞直接注射到兔肌肉组织后 ,皮肤成纤维细胞可以长期存活并持续表达外源基因 .其中β 半乳糖苷酶表达至少持续 3个月 ,人凝血因子Ⅸ蛋白表达持续 1个月 .研究结果将皮肤成纤维细胞的优点和肌肉组织途径的优势有机地结合起来 ,为血友病B及其他遗传病的体细胞基因治疗提供一条新的途径 .     

全身放射损伤对皮肤伤口成纤维细胞参与组织修复能力的影响

合并全身放射损伤的创伤（放创复合伤）是一种重要而有代表性的难愈性创伤,其难愈机制尚未完全阐明,成纤维细胞是最为重要的组织修复细胞,其辐射敏感性较低,为了明确放创复合伤时合并的放射损伤是否对伤口成纤维细胞有直接损伤作用,以及这些损伤作用对创伤愈合的影响,实验检测了分离,培养的放创复合伤和单纯创伤大鼠皮肤伤口成纤维细胞的增殖,凋亡及其他反映其参与组织修复能力的指标变化,结果发现,在去除全身因素和局部因素,特别是创伤局部细胞因子和细胞外基质对成纤维细胞的反馈作用后,放创复合伤组伤口成纤维细胞增殖力,贴壁力和粘附力均显著弱于单纯创伤组,而成纤维细胞的凋亡率则显著增加,这些细胞表明,全身放射损伤对伤口成纤维细胞有直接损伤作用,使其参与组织修复能力显著受抑,这是合并全身放射损伤时创伤难愈的重要原因。     

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。     

Adenyl Cyclase Activity in Cultivated Human Skin Fibroblasts

CYCLIC 3′,5′-AMP (cyclic AMP) is an important regulator of cellular processes^{1, 2}. In target cells, hormones stimulate adenyl cyclase, an enzyme which catalyses the conversion of ATP to cyclic AMP, which acts as a “second messenger” on either a membrane or an enzyme system and produces a specific physiological response. Hormonal stimulation of adenyl cyclase in several tissues has been documented².     

人皮肤成纤维细胞在不同培养系统中的生长代谢特性

大面积烧伤病人及多种皮肤溃疡病人很难用自体皮肤移植来进行治疗.早期治疗方法采用尸体来源的皮肤移植,但由于来源有限、且有传播疾病的危险,因此应用组织工程技术构建生物活性人工皮肤已成为近十几年来在组织工程和创伤治疗领域的研究热点,目前已有几种人工皮肤成功地走向临床[1].然而,在构建大面积皮肤组织过程中,如何大量制备皮肤种子细胞仍然是一大棘手的难题,成为人体皮肤组织工程迫切需要解决的技术关键.获得大量扩增的皮肤细胞,解决种子细胞的供应问题,是构建人工皮肤的一个关键.     

Growth Stimulation of Human Skin Fibroblasts by Elastin-Derived Peptides

Elastin-derived peptides (kappa-elastin: KE, mean molecular mass: 75 kDa), either coated onto plastic dishes or added to culture media (0.26 to 1.33 nM) stimulated the growth of human skin fibroblasts (HSF) strains obtained from different donors and tested at different cell passages (4 to 12). Coated 44.4 μg/cm²insoluble elastin (iE) exhibited the same action; coated iE or KE significantly modifies the HSF morphology: after 5-6 days of culture, HSF are more elongated, and at preconfluence state, formation of HSF clusters surrounding iE were observed. Increased ³H thymidine incorporation and proliferative effect of HSF by KE (1.3 to 2.2 fold as compared to control cells) was observed after a lag phase period which raised with initial HSF density. Optimal proliferative effect was obtained at KE 8.5 10^-10M, a value close to the dissociation constant (k_D= 2.7 10^-10M) of KE to HSF. Valine-glycine-valine-alanine-proline-glycine (VGVAPG), but not valine-glycine-valine (VGV) or Valine-glycine-valine-valine-glycine-alanine (VGWGA) also significantly stimulated, optimally at 7.0 10^-10M, HSF proliferation. It was concluded that the stimulatory influence of elastin derived peptides on HSF proliferation was mediated through a binding to plasmalemmal receptor of HSF.     

Growth Stimulation of Human Skin Fibroblasts by Elastin-Derived Peptides

Elastin-derived peptides (kappa-elastin: KE, mean molecular mass: 75 kDa), either coated onto plastic dishes or added to culture media (0.26 to 1.33 nM) stimulated the growth of human skin fibroblasts (HSF) strains obtained from different donors and tested at different cell passages (4 to 12). Coated 44.4 μg/cm²insoluble elastin (iE) exhibited the same action; coated iE or KE significantly modifies the HSF morphology: after 5-6 days of culture, HSF are more elongated, and at preconfluence state, formation of HSF clusters surrounding iE were observed. Increased ³H thymidine incorporation and proliferative effect of HSF by KE (1.3 to 2.2 fold as compared to control cells) was observed after a lag phase period which raised with initial HSF density. Optimal proliferative effect was obtained at KE 8.5 10^?10M, a value close to the dissociation constant (k_D= 2.7 10^?10M) of KE to HSF. Valine-glycine-valine-alanine-proline-glycine (VGVAPG), but not valine-glycine-valine (VGV) or Valine-glycine-valine-valine-glycine-alanine (VGWGA) also significantly stimulated, optimally at 7.0 10^?10M, HSF proliferation. It was concluded that the stimulatory influence of elastin derived peptides on HSF proliferation was mediated through a binding to plasmalemmal receptor of HSF.     

Dramatic Increase in Oxidative Stress in Carbon-Irradiated Normal Human Skin Fibroblasts

Skin complications were recently reported after carbon-ion (C-ion) radiation therapy. Oxidative stress is considered an important pathway in the appearance of late skin reactions. We evaluated oxidative stress in normal human skin fibroblasts after carbon-ion vs. X-ray irradiation. Survival curves and radiobiological parameters were calculated. DNA damage was quantified, as were lipid peroxidation (LPO), protein carbonylation and antioxidant enzyme activities. Reduced and oxidized glutathione ratios (GSH/GSSG) were determined. Proinflammatory cytokine secretion in culture supernatants was evaluated. The relative biological effectiveness (RBE) of C-ions vs. X-rays was 4.8 at D₀ (irradiation dose corresponding to a surviving fraction of 37%). Surviving fraction at 2 Gy (SF2) was 71.8% and 7.6% for X-rays and C-ions, respectively. Compared with X-rays, immediate DNA damage was increased less after C-ions, but a late increase was observed at D_10% (irradiation dose corresponding to a surviving fraction of 10%). LPO products and protein carbonyls were only increased 24 hours after C-ions. After X-rays, superoxide dismutase (SOD) activity was strongly increased immediately and on day 14 at D_0% (irradiation dose corresponding to a surviving fraction of around 0%), catalase activity was unchanged and glutathione peroxidase (GPx) activity was increased only on day 14. These activities were decreased after C-ions compared with X-rays. GSH/GSSG was unchanged after X-rays but was decreased immediately after C-ion irradiation before an increase from day 7. Secretion of IL-6 was increased at late times after X-ray irradiation. After C-ion irradiation, IL-6 concentration was increased on day 7 but was lower compared with X-rays at later times. C-ion effects on normal human skin fibroblasts seemed to be harmful in comparison with X-rays as they produce late DNA damage, LPO products and protein carbonyls, and as they decrease antioxidant defences. Mechanisms leading to this discrepancy between the two types of radiation should be investigated.     

化学发光法测定正常人皮肤纤维母细胞高密度脂蛋白(HDL)受体功能

A cbemiluminescence assay of human skin fibroblasts HDL receptor function was established.HDL3 was labelled with 6(N-(4-amino butyl)~N-ethyl)-amino-2,3-dihydro phthalazine l,4-dione(ABEI) by the carbodiimide(EDC).The labelled compound (HDL3-ABEI) was water soluble and non-toxic.It was stored at -30*********C before use.HDL3 was isolated by sequential ultracentrifugation.The HDL3 obtained was Apo-E-free.After incubation of HDL3 in waterbath at 52**********C for 3 hours, the HDL3 was labelled with ABEI to a ratio of 0.89 m mol ABEI/mmol HDL3.The HDL3-ABEI showed positive immunore action with antibodies of Apo A-********I and Apo A-*******II, indic-eting that the labelled HDL3 still retained its immunological characteristics.The conditions for determination of HDL receptor function of human skin fibroblasts were studied.The optimum quantity of HDL3-ABEI for combination with fibroblasts HDL receptors at 4癈 was 20********ug.The optimum time for combination of HDL3-ABEI with fibroblasts HDL receptors at 4*********C was 1 hour.The amount of HDL required for blocking HDL receptors was 400********ug.The optimum cell number for combination of HDL3-ABEI with HDL receptors was 1**********X105 cells/ml.In the mean time, the decrease in luminescence intensity with the increase in number of cells was observed.Again a high protein concentration would cause inhibition to the assay system.     

Skin Filling and Firming Activity of a Hyaluronic Acid Inducing Synthetic Tripeptide

International Journal of Peptide Research and Therapeutics - Aging of skin manifests in loss of volume and firming due to degradation of extracellular matrix components such as collagen and...     

Synthesis of Oligosaccharides Structurally Related to Hyaluronic Acid Fragments

Russian Journal of Bioorganic Chemistry - Hyaluronic acid (HA) is a natural polysaccharide constructed from the alternating residues of β-D-glucuronic acid and N-acetyl-β-D-glucosamine....     

Lactate Oxidation for the Detection of Mitochondrial Dysfunction in Human Skin Fibroblasts

To screen fibroblasts for defects in lactate/pyruvate oxidation, cells were grown to confluence in 25-cm² flasks, rinsed, and incubated in glucose-free media containing 25 μM L-lactate and 0.1 μCi [D,L-1-¹⁴C]lactate. Lactate oxidation was measured as the amount of lactate oxidized in nmol of ¹⁴CO₂ generated /mg protein/min. Fibroblasts from patients with mitochondrial or peroxisomal disorders had decreased lactate oxidation compared to the control (CON): CON, 1.9 ± 0.13 nmol/mg/min; neonatal adrenoleukodystrophy (NALD), 0.45 ± 0.01 (P < 0.001); rhizomelic chondrodysplasia punctata (RCDP), 0.13 ± 0.002 (P < 0.001); mitochondrial defect of unknown etiology (MIT), 0.77 ± 0.003 (P <0.001); pyruvate dehydrogenase (PDH) deficiency, 0.98 ± 0.02 (P < 0.001). This method is useful for screening fibroblasts for defects in lactate oxidation in patients with mitochondrial or peroxisomal disorders. Confirmation of the site of the defect may then be investigated with specific assays, e.g., PDH, in cellular homogenates: CON, 0.93 ± 0.02 nmol/mg/min; NALD, 0.55 ± 0.02; RCDP, 0.44 ± 0.02; MIT, 0.53 ± 0.03; PDH deficiency, 0.19 ± 0.02.