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Cloning and Characterization of Pseudomonas mucidolens Exoinulinase
Kwon, Young Man,Kim, Hwa Young,Choi, Yong Jin 한국미생물 · 생명공학회 2000 Journal of microbiology and biotechnology Vol.10 No.2
An exoinulinase (β-D-fructofuranosidase) gene was cloned by chromosome walking along the upstream region of the endoinulinase gene of Pseudomonas mucidolens isolated from soil. The exoinulinase gene consisted of an ORF of 1,506bp encoding a polypeptide of 501 amino acids with a deduced molecular weight of 55,000. The exoinulinase produced by the recombinant Escherichia coli DH5α strain was also purified to homogeneity as determined by SDSPAGE and a zymogram. The molecular weight of the purified exoinulinase according to both SDS-PAGE and gel filtration matched the deduced molecular weight of the protein described above, thereby indicating that the native form of the exoinulinase was a monomer. The purified enzyme hydrolyzed sucrose, raff nose, levan, in addition to inulin, with an S/I activity value of 2.0. Furthermore, no inulo-oligomers were liberated from the inulin substrate in the enzymatic reaction mixtures incubated for 90min at 55℃. Taken together, these results indicate that the purified β-D-fructofuranosidase was an exoinulinase. The pH and temperature optima of the exoinulinase were pH 6.0 and 55℃, respectively. The enzyme had no apparent requirement for a cofactor, and its activity was completely inactivated by Ag^+, Hg^2+ , and Zn^2+. Kinetic experiments gave K_m, V_max, and K_cat, values for inulin of 11.5mM, 18nM/s, and 72s^-1, respectively. The exoinulinase was fairly stable in broad pH conditions (pH 5-9), and at pH 6.0 it showed a residual activity of about 70% after 4h incubation at 55℃.
Saccharomyces cerevisiae에서 Zymomonas mobilis 유래 Levansucrase의 발현과 분비
임채권,김이경,김광현,김철호,이상기,남수완 한국생명과학회 2004 생명과학회지 Vol.14 No.3
Zymomonas mobilis 유래 levansucrase 유전자(levU)를 GAL1 promoter 하류에 연결시킨 pYES-levU와 GAL10 promoter 하류에 Kluyveromyces marxianus exoinulinase의 분비 신호서열(INU1 ss) 하류에 연결시킨 pYInu-levU를 각각 구축하였다. 이들 plasmid를 invertase 결손 변이주(suc2-$\Delta$9)인 S. cerevisiae SEY2102에 형질전환시켜 고활성 형질전환주를 선발하였다. 효모 형질전환주를 galactose 함유 배지로 배양한 결과, pYES-levU 함유 형질전환주인 경우 levansucrase의 총활성은 7.17U/ml이고, pYInu-levU 함유 형질전환주인 경우 6.61U/ml에 도달하였다. 발현된 levansucrase 약 50% 정도가 배지와 periplasmic space에 존재하였고, INU1 ss에 의한 분비효율 증가는 관찰할 수 없었다. 또한, 효모에서 발현된 재조합 levansucrase는 과당쇄화된 형으로 생산되는 것으로 보여진다. Levansucrase gene (levU) from Zymomonas mobilis was subcloned downstream of GALl promoter in pYES 2.0 and pYInu-AT [GALl0 promoter+exoinulinase signal sequence of Kluyveromyces marxianus], resulting pYES-levU and pYInu-levU, respectively. The two expression plasmids were introduced into an invertase-deficient strain, Saccharomyces cerevisiae SEY2102, and then transformants showing high activity of levansucrase were selected. When each yeast transformants was cultivated in medium containing galactose, the extracellular and intracellular activities of levansucrase reached about 7.17 U/㎖ with the strain harboring pYES-levU and 6.61 U/㎖ with the strain harboring pYInu-levU. It was found that about 50% of levansucrase were detected in the medium and periplasmic space, and exoinulinase signal sequence didn't enhance the secretion efficiency. Furthermore, the recombinant levansucrase expressed in yeast seems to be produced as a hyper-glycosylated form.
임명예,이진우,이재형,김연희,서진호,남수완,Lim, Myung-Ye,Lee, Jin-Woo,Lee, Jae-Hyung,Kim, Yeon-Hee,Seo, Jin-Ho,Nam, Soo-Wan 한국생명과학회 2007 생명과학회지 Vol.17 No.9
Kluyveromyces marxianus 유래의 exoinulinase (INU1) 분비 서열과 GAL10 promoter를 이용하여 Clostridium thermocellum endoglucanase A gene (celA)의 과발현과 분비 성능 검증연구를 수행하였다. 자체 분비 서열을 가지는 pYEG- CT1 과 INU1 분비 서열을 가지는 pYInu-CT1, 두개의 plasmid는 S. cer-evisiae SEY2102와 S. cerevisiae 2805에 각각 형질전환시켜 ur-acil이 결핍된 배지에서 선별하였다. celA gene 자체 분비 서열보다 INU1 분비 서열을 사용했을 때 발현량과 분비효율은 각각 약 $18{\sim}22%$ 와 11% 향상되었다. 이 중 361 unit/l의 발현율과 89%의 plasmid 안정성, 그리고 70%의 분비효율을 보인 S. cerevisiae 2805/pYinu-CT1 효모 형질전환체를 cellolose를 효과적으로 분해하는 재조합 효모 생균체로 선별하였다. Galactose 배지내에서 S. cerevisiae 2805/ pYInu-CT1의 발효조 회분배양 결과, 총발현량과 분비효율은 각각 418 unit/l 와 73% 로 나타났다. 또한 분비된 endoglucanase A는 분자량 100kDa 이상에서 활성 밴드를 보여, N-linked 당쇄부가에 의해 상당한 비율의 당쇄가 부가됨을 추측할 수 있었다. The secretory overexpression of Clostridium thermocellum endoglucanase A gene (celA) was examined in Saccharomyces cerevisiae using Kluyveromyces marxianus exoinulinase (INU1) signal sequence and GAL10 promoter. The two plasmids, pYEG-CT1 with its own signal sequence, and pYInu-CT1 with INU1 signal sequence were introduced to S. cerevisiae SEY2102 and S. cerevisiae 2805 host strains, respectively, and then each transformant was selected on the synthetic defined media lacking uracil. The expression level and secretion efficiency of endoglucanase A was increased by $18{\sim}22%$ and 11%, respectively, by INU1 signal sequence over celA signal sequence. By considering the high level of expression (361 unit/I), plasmid stability (89%), and secretion efficiency (70%), S. cerevisiae 2805 harboring plasmid pYInu-CT1 was selected as the opti-mal host vector system for the production of cellulose-degrading enzyme and recombinant yeast probiotic. The total expression and secretion efficiency of endoglucanase A was 418 unit/l and 73%, respectively, in the batch fermentation of S. cerevisiae 2805/pYlnu-CT1 on galactose medium. The mo-lecular weight of secreted endoglucanase A was found to be greater than 100 kDa, presumably due to the N-linked glycosylation.