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한호석,박정혜,최희진,손준호,김영활,김성,최청 한국식생활문화학회 2004 韓國食生活文化學會誌 Vol.19 No.1
The biochemical components of Namcheondlggae, Miryangdlkkae 25, Boradlggae and Ipdlkkae 1 were measured. The samples were extracted with hot water, 60% acetone or 80% ethanol for screening physiological activity. The crude protein content (4.36%) was found in the Miryangdlkkae 25 and calcium content (497.5 mg%) was found in the Namcheondlggae among the tested 4 perilla leaves. Fructose was 30.86 mg% in the Namcheondlggae and free amino acids at all perilla leaves was detected seventeen. In Boradlggae, glutamic acid and alanin were 25.37 and 11.91 mg%. Totally nine non-volatile organic acids were also detected and the contents of malic acid and glutaric acid were 28.34 and 14.57 mg% in Boradlggae. The Miryangdlkkae 25 had the highest vitamin C amount which was 113.24 mg%. Angiotensin converting enzyme (ACE) inhibition activity of 80% ethanol extract of Boradlggae was 46.71%. Electron donating activity of 60% acetone extract from Namcheondlggae was the strongest inhibition activity as 98.19% when 200ppm level of the sample extracts were added.
한국재래간장으로 부터 분리한 Bacillus subtilis CCKS-111이 생성하는 Protease의 분리 및 정제
김성,임성일,이희덕,이선호,손준호,최희진,김영활,최청,Kim, Sung,Lim, Seong-Il,Lee, Hee-Duck,Lee, Seon-Ho,Son, Jun-Ho,Choi, Hee-Jin,Kim, Yeung-Hweal,Choi, Cheong 한국응용생명화학회 1997 Applied Biological Chemistry (Appl Biol Chem) Vol.43 No.2
한국재래간장으로 부터 분리한 Bacilius subtilis CCKS-111이 생성하는 proteae를 분리 정제하였다. 황산암모늄 염석, DEAE cellulose ion-exchange chromatography, Sephades G-100 및 HPLC를 이용한 겔여과법에 의해 비활성도 24.3 unit/mg, 정제배수 50.6배로 효소를 정제하였으며 high performance liquid chromatography (HPLC)에 의하여 단일 단백질임을 확인하였다 정제효소의 분자량은 HPLC에 의하여 분자량 28,000 정도의 monomer로 추정되었고, 본 효소의 아미노산 잔기수는 251.3으로, 분해되기 쉬운 threonine, serine, glycine을 제외한 아미노산 잔기수는 Bacillus subtilis subtilisin DY 잔기수(274)와 유사한 것으로 나타났다. 아미노산 조성은 alanine, serine, glycine 및 arginine의 함량이 많았다. Reverse phase (RP)-HPLC로 분리한 주 peak로 N-말단에서 32번 까지 아미노산 배열을 확인한 결과 Bacillus subtilis subtilisin DY와 동일하였다. A protease was purified from Bacillus subtilis CCKS-111 by ammonium sulfate treatment, DEAE-cellulose ion-exchange chromatography, Sephadex G-100 gel filtration and high performance liquid chromatography (HPLC). The specific activity of the purified enzyme was 24.3 unit/mg protein and the purification fold of enzyme was 50.6. Molecular weight of the purified enzyme estimated about 28,000 by HPLC gel filtration. The amino acid residues of this enzyme were 251.3 except threonine, serine and glycine. This result was similar to Bacillus subtilis subtilisin DY. From the first N-terminal amino acid to the 32th amino acid, the amino acid sequence was estimated after RP-HPLC elution. N-terminal and the 32th amino acids were alanine and aspartic acid. Alanine, serine, glycine and arginine were four major acids in the enzyme.
한국재래간장으로 부터 분리한 Bacillus subtilis CCKS-111이 생성하는 Protease의 분리 및 정제
최청,김성,임성일,이희덕,이선호,손준호,최희진,김영활 ( Cheong Choi,Sung Kim,Seong Il Lim,Hee-Duck Lee,Seon Ho Lee,Jun Ho Son,Hee Jin Choi,Yeung hweal Kim ) 한국응용생명화학회 1997 Applied Biological Chemistry (Appl Biol Chem) Vol.40 No.3
A protease was purified from Bacillus subtilis CCKS-111 by ammonium sulfate treatment, DEAE-cellulose ion-exchange chromatography, Sephadex G-100 gel filtration and high performance liquid chromatography (HPLC). The specific activity of the purified enzyme was 24.3 unit/㎎ protein and the purification fold of enzyme was 50.6. Molecular weight of the purified enzyme estimated about 28,000 by HPLC gel filtration. The amino acid residues of this enzyme were 251.3 except threonine, serine and glycine. This result was similar to Bacillus subtilis subtilisin DY. From the first N-terminal amino acid to the 32th amino acid, the amino acid sequence was estimated after RP-HPLC elution. N-terminal and the 32th amino acids were alanine and aspartic acid. Alanine, serine, glycine and arginine were four major acids in the enzyme.