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人血清在支持人结膜上皮细胞体外和体内增殖中的应用。

The use of human serum in supporting the in vitro and in vivo proliferation of human conjunctival epithelial cells.

作者信息

Ang L P K, Tan D T H, Seah C J Y, Beuerman R W

机构信息

Singapore National Eye Center, 11 Third Hospital Avenue, Singapore 168751.

出版信息

Br J Ophthalmol. 2005 Jun;89(6):748-52. doi: 10.1136/bjo.2004.055046.

Abstract

AIM

To evaluate the use of human serum (HS) in supporting the in vitro and in vivo proliferation of human conjunctival epithelial cells, and compare it with fetal bovine serum (FBS) and bovine pituitary extract (BPE).

METHODS

Conjunctival epithelial cells were cultivated in media supplemented with HS (5%, 10%), FBS (5%, 10%), and BPE (70 microg/ml, 140 microg/ml). The colony forming efficiency (CFE), bromodeoxyuridine (BrdU) ELISA proliferation assay, and cell generations were analysed. Cells were evaluated for keratin (K4, K19, and K3) and MUC5AC expression by immunostaining and RT-PCR. Conjunctival equivalents constructed on amniotic membranes were transplanted onto severe combined immune deficient (SCID) mice for 10 days and analysed histologically.

RESULTS

The proliferation assays of HS supplemented cultures (CFE, 6.7% (SD 1.8%); BrdU absorbance, 0.86 (0.16)) were comparable to FBS supplemented (CFE, 9.3% (1.8%); BrdU absorbance, 1.11 (0.18)) and BPE supplemented cultures (CFE, 5.9 (1.5); BrdU absorbance, 0.65 (0.12)). Goblet cell densities for HS, FBS, and BPE supplemented media were 52 cells/cm(2), 60 cells/cm(2), and 50 cells/cm(2), respectively. HS supplemented cultures formed stratified epithelial sheets in vivo following transplantation.

CONCLUSIONS

The proliferative capacity of conjunctival epithelial cells cultivated in HS supplemented cultures was comparable to FBS and BPE supplemented cultures. The elimination of animal material from the culture system is advantageous when cultivating cells for clinical transplantation.

摘要

目的

评估人血清(HS)在支持人结膜上皮细胞体外和体内增殖方面的应用,并将其与胎牛血清(FBS)和牛垂体提取物(BPE)进行比较。

方法

结膜上皮细胞在补充有HS(5%、10%)、FBS(5%、10%)和BPE(70微克/毫升、140微克/毫升)的培养基中培养。分析集落形成效率(CFE)、溴脱氧尿苷(BrdU)ELISA增殖测定和细胞代次。通过免疫染色和逆转录-聚合酶链反应(RT-PCR)评估细胞对角蛋白(K4、K19和K3)和MUC5AC表达情况。在羊膜上构建的结膜替代物移植到严重联合免疫缺陷(SCID)小鼠上10天,并进行组织学分析。

结果

补充HS的培养物的增殖测定(CFE,6.7%(标准差1.8%);BrdU吸光度,0.86(0.16))与补充FBS的培养物(CFE,9.3%(1.8%);BrdU吸光度,1.11(0.18))和补充BPE的培养物(CFE,5.9(1.5);BrdU吸光度,0.65(0.12))相当。补充HS、FBS和BPE培养基的杯状细胞密度分别为52个细胞/平方厘米、60个细胞/平方厘米和50个细胞/平方厘米。移植后,补充HS的培养物在体内形成了分层上皮片。

结论

在补充HS的培养物中培养的结膜上皮细胞的增殖能力与补充FBS和BPE的培养物相当。在为临床移植培养细胞时,从培养系统中去除动物材料是有利的。

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