SHI Ling, LU Ge, LI Hong-xiao, et al. Electroacupuncture promotes expression of glutathione related regulatory enzymes in ovary tissue of rats with diminished ovarian reserve[J]. Acupuncture research, 2023, 48(4): 378-384.
DOI:
SHI Ling, LU Ge, LI Hong-xiao, et al. Electroacupuncture promotes expression of glutathione related regulatory enzymes in ovary tissue of rats with diminished ovarian reserve[J]. Acupuncture research, 2023, 48(4): 378-384. DOI: 10.13702/j.1000-0607.20211226.
Electroacupuncture promotes expression of glutathione related regulatory enzymes in ovary tissue of rats with diminished ovarian reserve
0.05)。结论:电针可调节DOR大鼠的动情周期,改善性激素水平,减轻机体氧化损伤程度,增加卵巢组织γ-GCS、GR蛋白及基因表达,提高肝脏GSH水平,提示电针可能通过调节卵巢GSH相关调控酶蛋白及mRNA表达,提高机体抗氧化应激能力,改善卵巢功能。Objective To observe the effect of electroacupuncture(EA) on ovarian function and expression of glutathione(GSH) related regulatory enzymes γ-glutamylcysteine synthetase(γ-GCS)
glutathione reductase(GR) protein and gene in rats with diminished ovarian reserve(DOR)
so as to explore its mechanisms underlying up-regulation of antioxidant stress ability. Methods A total of 30 female SD rats with normal estrous cycle were randomly divided into blank control
model and EA groups
with 10 rats in each group. The DOR model was established by gavage of tripterygium wilfordii polyglycoside suspension(50 mg·kg(-1))连续灌胃14 d复制DOR模型。电针组每日灌胃1 h后隔日交替电针双侧“肾俞”和“中脘”“关元”
Objective To observe the effect of electroacupuncture(EA) on ovarian function and expression of glutathione(GSH) related regulatory enzymes γ-glutamylcysteine synthetase(γ-GCS)
glutathione reductase(GR) protein and gene in rats with diminished ovarian reserve(DOR)
so as to explore its mechanisms underlying up-regulation of antioxidant stress ability. Methods A total of 30 female SD rats with normal estrous cycle were randomly divided into blank control
model and EA groups
with 10 rats in each group. The DOR model was established by gavage of tripterygium wilfordii polyglycoside suspension(50 mg·kg
(-1)
·d(-1)·d
(-1)
) for 14 consecutive days
while the rats in the blank group were given equal volume of 0.9% sodium chloride solution. One hour after daily gavage
EA(1.0 mA
100 Hz) was applied alternately to bilateral “Shenshu”(BL23)
and “Zhongwan”(CV12)+“Guanyuan”(CV4) for 10 min
for 14 consecutive days. Estrous cycles of rats in each group were observed and recorded daily during intervention.After the intervention
H.E.staining was used to observe histopathological changes of the ovarian tissue. The contents of serum sex hormones [follicle stimulating hormone(FSH)
anti-mullerian hormone(AMH)
estradiol(E_2)] and oxidative damage markers [8-hydroxydeoxyguanosine(8-OHDG) and nitrotyrosine(NTY)]
were determined by ELISA. The contents of GSH and oxidized glutathione(GSSG) in the liver tissue were determined by colorimetry
and their ratios were calculated. Immunohistochemistry and real-time fluorescence quantitative PCR were used to detect the immunoactivity and gene expression levels of γ-GCS and GR in the ovarian tissues
respectively. Results Compared with the blank group
the model group had a marked increase in the disorder rate of estrous cycle
serum FSH
8-OHDG and NTY contents(P
<
0.01) and a considerable decrease in the levels of serum AMH and E_2
liver GSH and GSSG contents and GSH/GSSG ratio
ovarian optical density and cell number as well as the expression of γ-GCS and GR mRNAs(P
<
0.05
P
<
0.01). After EA intervention
the increase of the disorder rate of estrous cycle
serum FSH
8-OHDG and NTY contents and the decrease of serum AMH and E_2
liver GSH and GSSG contents and GSH/GSSG ratio
ovarian optical density and cell number of γ-GCS and GR as well as the expression of γ-GCS genes were all reversed(P
<
0.01
P
<
0.05). H.E. staining showed degenerative changes of the ovarian tissue
fewer follicles at every level and increase of atretic follicles
disarrangement and layer number decrease of granulosa cells
and atrophy of corpus luteum in the model group
which were relatively milder in the EA group. Conclusion EA can improve ovarian function
and reduce oxidative stress damage in DOR rats
which may be associated with its functions in up-regulating the expression of γ-GCS and GR protein and gene in the ovarian tissue.
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