Jouve J L, Mottet V, Cottalorda J, Frayssinet P, Bollini G
Department of Pediatric Surgery, Hôpital Timone Enfants, Marseille, France.
J Pediatr Orthop B. 1998 Apr;7(2):167-73. doi: 10.1097/01202412-199804000-00016.
Growth plate lesions or resections may cause severe growth arrest because of the bony bridge between the epiphysis and metaphysis. Actual treatments for epiphysiodesis include resecting the bone bar and setting an interpositional material. Growth plate cultures may provide the appropriate cartilage necessary to restore growth potential when implanted in a growth plate defect. The aim of this work was to determine certain cell culture parameters in order to optimize in vitro cultures to obtain abundantly mature and functional chondrocytes. We studied the manner in which enzymatic digestion, carried out by various enzymes, obtained chondrocytes. Treatment with trypsin (0.2%) during 30 minutes at 37 degrees C and then collagenase (200 U/mL) during 6 hours was chosen. Under these conditions, 40 +/- 16 10(6) chondrocytes per gram of growth plate were obtained, and cellular viability was 79 +/- 12%. The density of the cellular seeding, the nature of the culture substrate, and the culture medium composition were determined to optimize the growth of differentiated cells. Seeding at 20,000 or 30,000/cm2 on a type I substrate and Ham F-12 medium not supplemented with either glucose or growth factors was demonstrated to be the best choice for this purpose.
生长板损伤或切除术可能会因骨骺与干骺端之间形成骨桥而导致严重的生长停滞。骺板固定术的实际治疗方法包括切除骨桥并植入间隔材料。生长板培养物在植入生长板缺损时,可能会提供恢复生长潜能所需的合适软骨。这项工作的目的是确定某些细胞培养参数,以优化体外培养,从而获得大量成熟且功能正常的软骨细胞。我们研究了用各种酶进行酶消化获取软骨细胞的方式。选择在37℃下用0.2%胰蛋白酶处理30分钟,然后用200 U/mL胶原酶处理6小时。在这些条件下,每克生长板可获得40±16×10⁶个软骨细胞,细胞活力为79±12%。为优化分化细胞的生长,我们确定了细胞接种密度、培养底物的性质以及培养基成分。结果表明,在此目的下,以每平方厘米20000或30000个细胞的密度接种于I型底物上,且不添加葡萄糖或生长因子的Ham F-12培养基是最佳选择。
