De S K, Enders G C, Andrews G K
Department of Biochemistry and Molecular Biology, University of Kansas Medical Center, Kansas City 66103.
Mol Endocrinol. 1991 May;5(5):628-36. doi: 10.1210/mend-5-5-628.
Northern blotting, in situ hybridization, and oligodeoxyribonucleotide excess solution hybridization were used to quantitate metallothionein-I (MT-I) and MT-II mRNAs in mouse testes. Testes from sexually mature adults contained high levels of both MT mRNAs (approximately 10-fold higher than those in control adult liver). Testicular MT mRNA levels were age dependent, being low the first 2 weeks after birth and increasing slowly thereafter to maximal levels in the adult (by 9 weeks after birth). In the adult testis, in situ hybridization indicated that only cells within the adluminal compartment (germ cells) of the seminiferous tubules contain high levels of MT mRNA. The appearance of cells containing elevated levels of MT mRNA during development was delayed from the onset of spermatogenesis. In situ hybridization suggested that MT mRNA accumulates after the initial differentiation of primary spermatocytes and is maintained in spermatids. Pachytene spermatocytes (PSC) and round spermatids (RTD) isolated from adult testes contained both MT-I and MT-II mRNAs in levels equivalent to those found in zinc-treated hepatocytes, whereas very low levels of MT mRNA were detected in isolated Sertoli cells (ST). In situ hybridization suggested that MT mRNA was present at only basal levels in interstitial, spermatogonial, and mature sperm cells at all developmental stages examined. Northern blot and in situ hybridization to sulfated glycoprotein-2 (SGP-2) mRNA, a ST-specific transcript, showed that SGP-2 mRNA is high in the testis of 1-week-old mice and decreases gradually to a lower level in the adult. In situ detection of this mRNA was consistent with the location of ST in the testis. SGP-2 mRNA was abundant in ST and rare in PSC and RTD preparations. Analysis of pulse-labeled proteins from isolated PSC and RTD indicated that these cells actively synthesize MT-I and MT-II. The high levels of MT mRNA in adult testes were not increased substantially after systemic injection of cadmium, zinc, or bacterial lipopolysaccharide. In marked contrast, these treatments led to dramatically increased levels of hepatic and ovarian MT mRNA. This study establishes that the MT genes are actively expressed in a developmentally regulated fashion in the male germ cells of the mouse. This suggests a role for MT in the process of spermatogenesis.
采用Northern印迹法、原位杂交法和寡脱氧核糖核苷酸过量溶液杂交法对小鼠睾丸中的金属硫蛋白-I(MT-I)和MT-II mRNA进行定量分析。性成熟成年小鼠的睾丸中这两种MT mRNA水平都很高(比对照成年肝脏中的水平高约10倍)。睾丸MT mRNA水平与年龄有关,出生后的前2周较低,此后缓慢上升,在成年期(出生后9周)达到最高水平。在成年睾丸中,原位杂交表明,只有生精小管管腔内侧隔室(生殖细胞)中的细胞含有高水平的MT mRNA。发育过程中MT mRNA水平升高的细胞出现时间比精子发生开始时间延迟。原位杂交表明,MT mRNA在初级精母细胞初步分化后积累,并在精子细胞中维持。从成年睾丸中分离出的粗线期精母细胞(PSC)和圆形精子细胞(RTD)中MT-I和MT-II mRNA水平与锌处理的肝细胞中的水平相当,而在分离的支持细胞(ST)中检测到的MT mRNA水平非常低。原位杂交表明,在所检查的所有发育阶段,MT mRNA仅在间质、精原细胞和成熟精子细胞中处于基础水平。对硫酸化糖蛋白-2(SGP-2)mRNA(一种ST特异性转录本)进行Northern印迹和原位杂交显示,SGP-2 mRNA在1周龄小鼠的睾丸中含量很高,在成年期逐渐降低至较低水平。该mRNA的原位检测结果与ST在睾丸中的位置一致。SGP-2 mRNA在ST中丰富,在PSC和RTD制剂中稀少。对分离的PSC和RTD中脉冲标记蛋白的分析表明,这些细胞能活跃地合成MT-I和MT-II。全身注射镉、锌或细菌脂多糖后,成年睾丸中高水平的MT mRNA没有显著增加。与之形成鲜明对比的是,这些处理导致肝脏和卵巢MT mRNA水平显著升高。本研究证实,MT基因在小鼠雄性生殖细胞中以发育调控的方式活跃表达。这表明MT在精子发生过程中发挥作用。
