小鼠次生卵泡在特定合成基质中的体外三维培养

Md. Asaduzzman, X. Cui, Hu Zhang, F. Young
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引用次数: 6

摘要

卵巢卵泡在体外三维(3D)基质中生长存在局限性:a)基质不随卵泡生长而膨胀,b)需要酶介导的检索,c)动物源性成分妨碍临床应用。因此,我们评估了n -异丙基丙烯酰胺(SFX-1),一种新的合成3D培养基质,用于卵泡培养。将3组小鼠次级卵泡包埋于50 μL DMEM/F12-1% its -10% fcs (DMEM/F12)或SFX-1 (3:2 v/v DMEM/F12)或Matrigel (1:1 DMEM/F12)中,培养48 h。Matrigel含有生长因子,SFX-1不含动物源性因子。每种培养条件分别在6个含有18个卵泡的孔中进行4次重复实验(n = 4)。利用显微照片测定卵泡直径和形态完整性。对卵泡进行活死(LD)染色或分解,生成细胞,用台盼蓝(TB)进行活力评估。采用酶联免疫法测定条件培养基中的雌二醇、黄体酮和抗苗勒管激素(AMH)。所有培养条件都支持类似的卵泡直径增加。DMEM/F12未保持形态完整性,导致48 h后无法取出卵泡;从DMEM/F12中提取25%的卵泡,从SFX-1和Matrigel中分别提取44%和41%的卵泡。从Matrigel提取的卵泡不能分解,这阻碍了结核病生存能力的评估。活细胞/卵泡的LD值低于TB,但培养条件对活细胞/卵泡的存活率没有影响;SFX-1 64%±8%,DMEM/F12 69%±9%。SFX-1和Matrigel支持相似水平的黄体酮合成,只有Matrigel支持雌激素合成,但没有培养条件支持AMH的产生。SFX-1无细胞毒性,与Matrigel相当。支持SFX-1用于人类卵泡的进一步开发。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Three Dimensional In Vitro Culture of Murine Secondary Follicles in a Defined Synthetic Matrix
Ovarian follicle growth in three dimensional (3D) matrices in vitro has limitations: a) matrices don’t expand as follicles grow, b) requirements for enzyme-mediated retrieval, and c) animal-derived components prevent clinical application. Therefore, we evaluated N-Isopropylacrylamide (SFX-1), a novel synthetic 3D culture matrix, for follicle culture. Groups of three murine secondary follicles were encapsulated in 50 μL of DMEM/F12-1%ITS-10%FCS (DMEM/F12) or SFX-1 (3:2 v/v DMEM/F12) or Matrigel (1:1 DMEM/F12) and cultured for 48 h. Matrigel contains growth factors but SFX-1 has no animal-derived factors. Each culture condition was examined in 6 wells containing 18 follicles, in four replicate experiments (n = 4). Photomicrographs were used to determine follicle diameters and morphological integrity. Follicles were Live-Dead (LD) stained or disaggregated to generate cells for viability assessment using Trypan Blue (TB). Estradiol, progesterone and anti-mullerian hormone (AMH) in conditioned media were measured using Enzyme-linked Immunoassay. All culture conditions supported similar increases in follicle diameter. DMEM/F12 did not maintain morphological integrity which prevented follicle retrieval after 48 h; 25% were retrieved from DMEM/F12, but 44% and 41% follicles were retrieved from SFX-1 and Matrigel respectively. Follicles retrieved from Matrigel could not be disaggregated, which prevented TB viability assessment. LD estimations of viable cells/follicle were lower than TB, but culture conditions had no effect on viability; SFX-1 64% ± 8% and DMEM/F12 69% ± 9%. SFX-1 and Matrigel supported similar levels of progesterone synthesis, only Matrigel supported estrogen synthesis, but none of the culture conditions supported AMH production. SFX-1 was not cytotoxic and was comparable to Matrigel. Further development of SFX-1 for use with human follicles is supported.
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