Purification and subfractionation of bovine thyrotropin and lutropin using radioimmunoassays for evaluation of the purification processes

Procedures for the group separation of bovine pituitary glycoprotein hormones, i.e., thyrotropin, lutropin, and follitropin, and for the purification and subfractionation of the first two hormones were studied. Radioimmunoassay systems specific to bovine thyrotropin and lutropin have been developed...

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Published inJournal of biochemistry (Tokyo) Vol. 83; no. 4; pp. 1173 - 1190
Main Authors Yora, T, Ui, N. (Gunma Univ., Maebashi (Japan). Inst. of Endocrinology)
Format Journal Article
LanguageEnglish
Published England Oxford University Press 01.04.1978
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Abstract Procedures for the group separation of bovine pituitary glycoprotein hormones, i.e., thyrotropin, lutropin, and follitropin, and for the purification and subfractionation of the first two hormones were studied. Radioimmunoassay systems specific to bovine thyrotropin and lutropin have been developed and used to evaluate these purification processes. Pituitary glycoprotein hormones were fractionally extracted with aqueous ethanol from 400 g of bovine lyophilized pituitary powder by the percolation method and purified by bioaffinity chromatog-raphy on a column of concanavalin A-Sepharose; more than 500-fold purification was achieved within 4-5 days and the estimated overall yield was close to 90% of the total extractable hormones. A mixture of thyrotropin and lutropin was obtained efficiently from this glycoprotein hormone concentrate by CM-cellulose chromatography and further fractionated by DEAE-cellulose chromatography. Although most of the lutropin was separated from thyrotropin on this chromatography, thyrotropin was always accompanied by a substantial amount of lutropin. On isoelectric focusing of the thyrotropin-containing fraction thus obtained, five peaks of immunologic thyrotropin with isoelectric points at pH 7.20, 7.90, 8.32, 8.60, and 8.95 were obtained; contaminating lutropin was also distributed over this pH range. Thyrotropin components completely free of lutropin could be obtained by the use of affinity chromatography on a column of immobilized anti-bovine lutropin antibodies. On the other hand, four components of bovine lutropin, completely or almost completely free of thyrotropin, were purified by isoelectric focusing of two lutropin fractions obtained by DEAE-celluIose chromatography. Their isoelectric points were distributed over a pH range of 8.2-9.0.
AbstractList Procedures for the group separation of bovine pituitary glycoprotein hormones, i.e., thyrotropin, lutropin, and follitropin, and for the purification and subfractionation of the first two hormones were studied. Radioimmunoassay systems specific to bovine thyrotropin and lutropin have been developed and used to evaluate these purification processes. Pituitary glycoprotein hormones were fractionally extracted with aqueous ethanol from 400 g of bovine lyophilized pituitary powder by the percolation method and purified by bioaffinity chromatog-raphy on a column of concanavalin A-Sepharose; more than 500-fold purification was achieved within 4-5 days and the estimated overall yield was close to 90% of the total extractable hormones. A mixture of thyrotropin and lutropin was obtained efficiently from this glycoprotein hormone concentrate by CM-cellulose chromatography and further fractionated by DEAE-cellulose chromatography. Although most of the lutropin was separated from thyrotropin on this chromatography, thyrotropin was always accompanied by a substantial amount of lutropin. On isoelectric focusing of the thyrotropin-containing fraction thus obtained, five peaks of immunologic thyrotropin with isoelectric points at pH 7.20, 7.90, 8.32, 8.60, and 8.95 were obtained; contaminating lutropin was also distributed over this pH range. Thyrotropin components completely free of lutropin could be obtained by the use of affinity chromatography on a column of immobilized anti-bovine lutropin antibodies. On the other hand, four components of bovine lutropin, completely or almost completely free of thyrotropin, were purified by isoelectric focusing of two lutropin fractions obtained by DEAE-celluIose chromatography. Their isoelectric points were distributed over a pH range of 8.2-9.0.
Author Yora, T
Ui, N. (Gunma Univ., Maebashi (Japan). Inst. of Endocrinology)
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1 This study was supported in part by a Scientific Research Grant (No. 121432) from the Ministry of Eduaction, Science and Culture of Japan.
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SubjectTerms Amino Acids - analysis
Animals
Cattle
Chromatography, Affinity
Chromatography, Ion Exchange
Follicle Stimulating Hormone - isolation & purification
Glycoproteins - isolation & purification
Isoelectric Focusing
Luteinizing Hormone - analysis
Luteinizing Hormone - isolation & purification
Pituitary Gland - analysis
Radioimmunoassay
Thyrotropin - analysis
Thyrotropin - isolation & purification
Title Purification and subfractionation of bovine thyrotropin and lutropin using radioimmunoassays for evaluation of the purification processes
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