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Tocotrienol preserves ovarian function in cyclophosphamide therapy
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Introduction:
Cyclophosphamide (CPA) chemotherapy leads to ovarian failure and infertility. Tocotrienol (T3) is an antioxidant and anti-inflammatory agent. The role of T3 in ovarian protection throughout chemotherapy remains unclear.
Aim:
To investigate the role of T3 in the preservation of female fertility in CPA treatment.
Method:
Sixty female mice were divided into five treatment groups, namely, normal saline, corn oil only, T3 only, CPA and CPA + T3. The treatment was given for 30 days, followed by administration of gonadotrophin to induce ovulation. After killing, both ovaries were collected and examined histologically.
Results:
There was significant reduction in ovarian size in the CPA group compared with the normal group (CPA versus normal, mean area ± SD; 0.118 ± 0.018 vs. 0.423 ± 0.024 cm
2
; p ≤ 0.005), whilst concurrent administration of T3 with CPA leads to conservation of ovarian size (CPA + T3 vs. CPA, mean area ± SD; 0.285 ± 0.032 vs. 0.118 ± 0.018 cm
2
; p ≤ 0.005). Ovaries in CPA group showed abnormal folliculogenesis with accompanied reduced ovulation rate, follicular oedema, increased vascularity and inflammatory cell infiltration. These changes were reversed by concurrent T3 administration.
Conclusion:
Co-administration of T3 with CPA confers protection of ovarian morphology and function in vivo. These findings contribute to the further elucidation of CPA effect on ovary and suggest the potential of T3 use in preserving fertility in chemotherapy.
Title: Tocotrienol preserves ovarian function in cyclophosphamide therapy
Description:
Introduction:
Cyclophosphamide (CPA) chemotherapy leads to ovarian failure and infertility.
Tocotrienol (T3) is an antioxidant and anti-inflammatory agent.
The role of T3 in ovarian protection throughout chemotherapy remains unclear.
Aim:
To investigate the role of T3 in the preservation of female fertility in CPA treatment.
Method:
Sixty female mice were divided into five treatment groups, namely, normal saline, corn oil only, T3 only, CPA and CPA + T3.
The treatment was given for 30 days, followed by administration of gonadotrophin to induce ovulation.
After killing, both ovaries were collected and examined histologically.
Results:
There was significant reduction in ovarian size in the CPA group compared with the normal group (CPA versus normal, mean area ± SD; 0.
118 ± 0.
018 vs.
0.
423 ± 0.
024 cm
2
; p ≤ 0.
005), whilst concurrent administration of T3 with CPA leads to conservation of ovarian size (CPA + T3 vs.
CPA, mean area ± SD; 0.
285 ± 0.
032 vs.
0.
118 ± 0.
018 cm
2
; p ≤ 0.
005).
Ovaries in CPA group showed abnormal folliculogenesis with accompanied reduced ovulation rate, follicular oedema, increased vascularity and inflammatory cell infiltration.
These changes were reversed by concurrent T3 administration.
Conclusion:
Co-administration of T3 with CPA confers protection of ovarian morphology and function in vivo.
These findings contribute to the further elucidation of CPA effect on ovary and suggest the potential of T3 use in preserving fertility in chemotherapy.
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