4.7 Article

Feasibility of Secondary Follicle Isolation, Culture and Achievement of In-Vitro Oocyte Maturation from Superovulated Ovaries: An Experimental Proof-of-Concept Study Using Mice

Journal

JOURNAL OF CLINICAL MEDICINE
Volume 10, Issue 13, Pages -

Publisher

MDPI
DOI: 10.3390/jcm10132757

Keywords

female fertility preservation; superovulation; follicle isolation; secondary follicle culture; in-vitro maturation; ovarian tissue

Funding

  1. Swedish Childhood Cancer Foundation [PR2016-0115, PR2020-0136]
  2. Swedish Cancer Society [CAN 2017/704, 20 0170 F]
  3. Swedish Research Council [2020-02230]
  4. Radiumhemmets Research Funds Grant for clinical researchers 2020-2025
  5. Stockholm County Council [FoUI-953912]
  6. Karolinska Institutet [2020-00339]
  7. China Scholarship Council
  8. Swedish Research Council [2020-02230] Funding Source: Swedish Research Council

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Experimental study showed that secondary follicles isolated from ovaries of mice treated with gonadotropins could be cultured in vitro and mature, with development and maturation abilities similar to those from unstimulated controls.
Fertility preservation through ovarian stimulation, aiming at cryopreserving mature oocytes or embryos, is sometimes unsuccessful. This clinical situation deserves novel approaches to overcome infertility following cancer treatment in patients facing highly gonadotoxic treatment. In this controlled experimental study, we investigated the feasibility of in-vitro culturing secondary follicles isolated from superovulated ovaries of mice recently treated with gonadotropins. The follicle yields of superovulated ovaries were 45.9% less than in unstimulated controls. Follicles from superovulated ovaries showed faster growth pace during the initial 7 days of culture and secreted more 17 beta-estradiol by the end of culture vs controls. Parameters reflecting the outcome of follicular development and oocyte maturation competence in vitro were similar between superovulated and control groups, with a similar follicle size at the end of culture and around 70% survival. Nearly half of cultured follicles met the criteria for in-vitro maturation in both groups and approximately 60% of those achieved a mature MII oocyte, similarly in both groups. Over 60% of obtained MII oocytes displayed normal-looking spindle and chromosome configurations, without significant differences between the groups. Using a validated follicle culture system, we demonstrated the feasibility of secondary follicle isolation, in-vitro culture and oocyte maturation with normal spindle and chromosome configurations obtained from superovulated mice ovaries.

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