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RESEARCH ARTICLE
Contents Vol 24(1)

121 ALGINATE-FIBRIN GEL MATRIX PROMOTES IN VITRO GROWTH OF DOG SECONDARY FOLLICLES

N. Songsasen A , C. Guzy A and D. E. Wildt A
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Smithsonian Conservation Biology Institute, Front Royal, VA, USA

Reproduction, Fertility and Development 24(1) 173-173 https://doi.org/10.1071/RDv24n1Ab121
Published: 6 December 2011

Abstract

A previous study from our laboratory has demonstrated that preantral follicles from the dog that are cultured in alginate are able to grow and produce steroid hormones (Songsasen et al. 2011 Reproduction 142, 113–122). Here we investigated the influence of using a combination of alginate and a degradable biomaterial, fibrin, on dog follicle development in vitro. We hypothesised that the alginate and fibrin gel matrix would be superior to alginate alone because the former has dynamic mechanical properties that permit more expansive follicle development than the inert alginate-only system. Secondary follicles (128–220 μm in diameter) were collected from the ovaries of 4 prepubertal dogs (<6 months of age) and encapsulated in 0.5% alginate (n = 26) or 0.5% alginate + 12.5 mg mL–1 of fibrin (n = 22). Follicles were cultured for 12 days at 38.5°C in 100 μL of α-minimal essential medium + 2 mM of glutamine + 5.5 μg mL–1 of insulin + 5.5 μg mL–1 of transferrin + 6.7 ng mL–1 of selenium + 10 μg mL–1 of FSH and 1 ng mL–1 of LH + 3 mg mL–1 of polyvinyl alcohol. Follicle diameter was monitored and half of the medium exchanged every 48 h. Follicle survival was assessed based on ability to increase in size, as well as on oocyte and granulosa cell morphology. Comparisons of follicle growth rate for each culture day between the 2 treatments were conducted using Student's t-test and among culture days within the same group using ANOVA followed by a Holm-Sidak multiple comparison. Follicle survival was compared using a chi-square test. In both groups, follicles maintained the 3-dimensional structure and increased (P < 0.05) in size as culture period progressed. However, follicles encapsulated in alginate + fibrin grew larger (P < 0.05) than those in alginate alone. Specifically, follicles in alginate + fibrin were doubled in size by 12 days compared with a 60% increase for alginate alone. There were no differences (P > 0.05) in follicle survival between the 2 groups (27.0 and 38.1% for alginate and alginate-fibrin, respectively). Results demonstrate that a dynamic alginate-fibrin matrix enhances in vitro follicle growth. We suspect that the mechanism involved is related to facilitating expansion capacity. Specifically, it is likely that nondegradable alginate offers physical, but eventually restrictive, support to encapsulated cells. By contrast, in the gel combination, the fibrin degrades due to cell-secreted proteases that, in turn, permit more robust follicle expansion. Low follicle survival (<40%) in both treatments emphasises the need for more studies to identify influential endocrine/paracrine factors that enhance follicle growth and production of competent oocytes.

Funded by NIH-KO1RR020564.