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成人隐静脉内皮细胞:评估其用于血管假体内皮种植的增殖能力。

Adult human saphenous vein endothelial cells: assessment of their reproductive capacity for use in endothelial seeding of vascular prostheses.

作者信息

Watkins M T, Sharefkin J B, Zajtchuk R, Maciag T M, D'Amore P A, Ryan U S, Van Wart H, Rich N M

出版信息

J Surg Res. 1984 Jun;36(6):588-96. doi: 10.1016/0022-4804(84)90145-8.

Abstract

Autogenous endothelial seeding (AES) of vascular prostheses (VP) using venous endothelial cells (EC) reduces platelet-VP interactions and improves patency rates in small caliber VP in dogs. To conserve patients' veins for use in coronary or limb bypass surgery, human trials of AES should require proof that adequate numbers of EC with the growth capacity to cover VP can be harvested from acceptably small pieces of peripheral vein. EC were isolated from excess saphenous vein segments remaining after coronary bypass surgery by filling veins with 0.1% CLS II collagenase at 37 degrees C for 15 min and removing EC by flushing the veins with culture medium. EC were cultured on fibronectin-coated dishes in medium 199 with 30% human serum and 300 micrograms/ml of endothelial cell growth factor. These cells grew to form confluent monolayers, and were identified as EC by tests for factor VIII antigen. Veins from 53 patients with a mean age of 55.8 +/- 9.8 (SD) years yielded vein segments with an average area of 1.9 +/- 0.6 cm2, from which an average of 5.3 +/- 2.8 X 10(4) cells were removed per cm2 of vein area. EC in culture underwent 14.3 +/- 1.4 population doublings with an average population doubling time of 1.8 +/- 0.3 days (N = 14 cultures), which allowed an 100-fold increase in cell number to occur in 11 to 12 days. These data suggest that the EC available from small vein segments in adult humans have the growth capacity to cover areas comparable in size to the luminal areas of VP commonly used in arterial surgery.

摘要

利用静脉内皮细胞对血管假体进行自体内皮接种(AES)可减少血小板与血管假体的相互作用,并提高犬类小口径血管假体的通畅率。为了保留患者的静脉用于冠状动脉或肢体搭桥手术,AES的人体试验应要求证明能够从足够小的外周静脉片段中获取数量充足且具有覆盖血管假体生长能力的内皮细胞。通过在37℃下用0.1% CLS II胶原酶填充静脉15分钟,然后用培养基冲洗静脉以去除内皮细胞,从冠状动脉搭桥手术后剩余的多余大隐静脉段中分离内皮细胞。内皮细胞在涂有纤连蛋白的培养皿中,于含有30%人血清和300微克/毫升内皮细胞生长因子的199培养基中培养。这些细胞生长形成汇合单层,并通过因子VIII抗原检测被鉴定为内皮细胞。53例平均年龄为55.8±9.8(标准差)岁的患者的静脉产生的静脉段平均面积为1.9±0.6平方厘米,每平方厘米静脉面积平均可去除5.3±2.8×10⁴个细胞。培养的内皮细胞经历了14.3±1.4次群体倍增,平均群体倍增时间为1.8±0.3天(N = 14个培养物),这使得细胞数量在11至12天内增加100倍。这些数据表明,成年人体内小静脉段中的内皮细胞具有生长能力,能够覆盖与动脉手术中常用血管假体管腔面积相当的区域。

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