4.7 Article

A two-step serum-free culture system supports development of human oocytes from primordial follicles in the presence of activin

Journal

HUMAN REPRODUCTION
Volume 23, Issue 5, Pages 1151-1158

Publisher

OXFORD UNIV PRESS
DOI: 10.1093/humrep/den070

Keywords

ovarian cortical strips; primordial follicle; preantral follicle; activin; in vitro oocyte culture

Funding

  1. Biotechnology and Biological Sciences Research Council Funding Source: Medline

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BACKGROUND: The objective of this study was to determine whether follicles grown within human ovarian cortical strip culture for 6 days in serum-free medium could be isolated at the secondary stage of pre-antral development and grown in vitro to the late pre-antral/early antral stage during a 4 day culture period. METHODS: Ovarian cortical biopsies were obtained from six women aged 26-40 years, with informed consent, during elective Caesarean section. Small tissue slices of ovarian cortex, with underlying stromal tissue removed, were cultured in serum-free medium for 6 days and at the end of this period pre-antral (secondary) follicles were dissected from the strips. Seventy-four intact pre-antral follicles ranging in size (66-132 mu m) (mean size 100 mu m +/- 3.4) were selected for further culture. Follicles were placed individually within V-shaped microwell culture plates in serum-free medium in the presence (n = 38) or absence (n = 36) of 100 ng/ml of human recombinant activin A. RESULTS: Pre-antral follicles grown for 4 days in the presence of activin A grew to a larger size (mean diameter 143 mu m +/- 7.4) than those grown in control medium (mean diameter 111 mu m +/- 8) (P < 0.005). Ninety percent of follicles cultured in the presence of activin A increased in size during the first 2 days of culture compared with only 36% of follicles in control medium (P > 0.005). Of the follicles surviving the entire culture period, 30% of those cultured in the presence of activin A showed normal morphology with intact oocytes and antral formation. None of the follicles grown in control medium developed antral cavities and > 90% of those follicles collected at the end of the culture period showed signs of oocyte degeneration. CONCLUSIONS: The results reported here demonstrate that under certain conditions, it is possible to achieve accelerated oocyte/follicle development from human primordial/primary follicles. This provides the first encouraging step towards achieving full in vitro growth of human oocytes.

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