转化核蛋白1作为受精失败患者的新生物标志物。

IF 1.8 Q3 OBSTETRICS & GYNECOLOGY
Jamileh Sadat Mirsanei, Hadis Gholipour, Zahra Zandieh, Masoumeh Golestan Jahromi, Mojgan Javedani Masroor, Mehdi Mehdizadeh, Fatemehsadat Amjadi
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引用次数: 0

摘要

目的:尽管卵胞浆内单精子注射(ICSI)是处理体外受精失败的一种方法,但仍有3%的夫妇在尝试ICSI后重复受精失败,尽管精子参数正常。这些患者是一个具有挑战性的群体,他们的精子在ICSI中不能使卵子受精。不幸的是,没有任何测试可以预测受精失败的风险。磷脂酶Cζ (PLCζ)和过渡核蛋白(TNPs)是精子成熟过程中染色质包装的重要因素。本研究旨在探讨plc - ζ1和TNP1在受精失败患者精子中的表达,以及DNA片段化指数、plc - ζ1和TNP1基因及蛋白表达与受精失败风险的相关性。方法:本研究选取12对受精率低的不育夫妇(结果:受精失败组DNA断裂率明显高于受精率组)。qRT-PCR和Western blot结果显示,这些患者的PLCζ和TNP1基因及蛋白表达明显低于对照组。结论:正常精子男性受精失败可能与DNA包装和TNP1表达不足有关。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

Transition nuclear protein 1 as a novel biomarker in patients with fertilization failure.

Transition nuclear protein 1 as a novel biomarker in patients with fertilization failure.

Transition nuclear protein 1 as a novel biomarker in patients with fertilization failure.

Transition nuclear protein 1 as a novel biomarker in patients with fertilization failure.

Objective: Although intracytoplasmic sperm injection (ICSI) is a way to deal with in vitro fertilization failure, 3% of couples still experience repeated fertilization failure after attempted ICSI, despite having sperm within normal parameters. These patients are a challenging group whose sperm cannot fertilize the egg during ICSI. Unfortunately, no test can predict the risk of fertilization failure. Phospholipase C zeta (PLCζ) and transition nuclear proteins (TNPs) are essential factors for chromatin packaging during sperm maturation. This study aimed to assess PLCζ1 and TNP1 expression in the sperm of patients with fertilization failure and the correlations among the DNA fragmentation index, PLCζ1 and TNP1 gene and protein expression, and the risk of fertilization failure.

Methods: In this study, 12 infertile couples with low fertilization rates (<25%) and complete failure of fertilization in their prior ICSI cycles despite normal sperm parameters were chosen as the case group. Fifteen individuals who underwent ICSI for the first time served as the control group. After sperm analysis and DNA fragmentation assays, quantitative reverse-transcription polymerase chain reaction (qRT-PCR) and Western blot analyses were performed to compare the gene and protein expression of PLCζ and TNP1 in both groups.

Results: DNA fragmentation was significantly higher in the fertilization failure group. The qRT-PCR and Western blot results demonstrated significantly lower PLCζ and TNP1 gene and protein expression in these patients than in controls.

Conclusion: The present study showed that fertilization failure in normozoospermic men was probably due to deficient DNA packaging and expression of TNP1.

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