Cox F, Gestautas J, Rapoport B
Department of Medicine, Veterans Administration Medical Center, San Francisco, California.
J Biol Chem. 1988 May 25;263(15):7060-7.
A lambda gt11 cDNA library was constructed using poly(A)+ mRNA from thyrotropin (TSH)-stimulated Fisher rat thyroid (FRTL5) cells. The library was screened for nonthyroglobulin cDNA sequences by differential plaque filter hybridization using single-stranded cDNA probes synthesized from mRNA prepared from quiescent and TSH-stimulated FRTL5 cells. Thyroglobulin cDNA-containing recombinants in the library were avoided by prehybridizing the TSH probe to excess thyroglobulin cDNA. Of 48,000 clones screened, 60 were chosen as representing mRNA species whose abundance was increased in TSH-stimulated versus quiescent cultures. Southern blot analysis of 9 clones confirmed that the TSH-cDNA probe hybridized to a greater extent to the cDNA inserts than did the control probe. cDNA insert sizes varied between 0.3 kilobase (kb) and 1.0 kb. Northern slot blot analysis using as probes the cDNA of four of these clones (FC4, FC26, FC29, and FC43) demonstrated that TSH stimulation of FRTL5 cells increased the steady state levels of the respective mRNA species by 4-12-fold. For all 4 clones, increases in mRNA levels were apparent within approximately 1 h and were maximal after 14-18 h of TSH stimulation. Determination of the partial nucleotide sequence of these 4 clones confirmed that none was thyroglobulin, thyroid peroxidase, or any other gene previously reported to be stimulated by TSH. Three of the clones bore no homology to any known nucleotide sequence, but FC26 was 85% homologous with human ferritin H. Northern blot analysis using the FC26 cDNA insert as a probe confirmed hybridization to an mRNA species of 1 kb, the known size of ferritin H mRNA. In summary, using the technique of differential plaque filter hybridization, we have identified 4 new genes whose mRNA levels are increased by TSH stimulation of thyroid cells. One of these genes is homologous to human ferritin H.
使用来自促甲状腺激素(TSH)刺激的Fisher大鼠甲状腺(FRTL5)细胞的聚腺苷酸加尾(poly(A)+)mRNA构建了λgt11 cDNA文库。通过差异噬菌斑滤膜杂交筛选该文库中的非甲状腺球蛋白cDNA序列,使用从静止和TSH刺激的FRTL5细胞制备的mRNA合成的单链cDNA探针。通过将TSH探针与过量的甲状腺球蛋白cDNA预杂交,避免文库中含甲状腺球蛋白cDNA的重组体。在筛选的48,000个克隆中,选择了60个作为代表在TSH刺激的培养物与静止培养物中丰度增加的mRNA种类。对9个克隆的Southern印迹分析证实,TSH-cDNA探针与cDNA插入片段的杂交程度比对照探针更大。cDNA插入片段大小在0.3千碱基(kb)至1.0 kb之间变化。使用其中四个克隆(FC4、FC26、FC29和FC43)的cDNA作为探针进行Northern印迹槽杂交分析表明,TSH刺激FRTL5细胞使各自mRNA种类的稳态水平增加了4至12倍。对于所有4个克隆,mRNA水平的增加在约1小时内明显,并在TSH刺激14至18小时后达到最大值。测定这4个克隆的部分核苷酸序列证实,没有一个是甲状腺球蛋白、甲状腺过氧化物酶或任何先前报道受TSH刺激的其他基因。其中三个克隆与任何已知核苷酸序列无同源性,但FC26与人类铁蛋白H有85%的同源性。使用FC26 cDNA插入片段作为探针的Northern印迹分析证实与1 kb的mRNA种类杂交,这是铁蛋白H mRNA的已知大小。总之,使用差异噬菌斑滤膜杂交技术,我们鉴定了4个新基因,其mRNA水平在甲状腺细胞受TSH刺激时增加。其中一个基因与人类铁蛋白H同源。
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