• 제목/요약/키워드: shaking-culture

검색결과 259건 처리시간 0.022초

Phellinus igniarius로부터 분리한 단백다당류의 분리 및 특성 (Characteristics and purification of proteoglycan from Phellinus igniarius)

  • 김선희;정인창;권용일;김소연;이종숙;이항우;이재성
    • Applied Biological Chemistry
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    • 제43권1호
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    • pp.57-62
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    • 2000
  • Phellinus igniarius의 배양방법별 균사체 및 단백다당류 생산수율비교 실험에서는 균사체내 다당류의 경우 모두 진탕배양이 효과적이었으나 균사체외 다당류의 경우 다당류 생산에서는 정치배양이 효과적이었다. 다당류의 정제는 조단백다당류를 이용하여 DEAE-cellulose column에 의한 1차 정제를 행하였고, 최종으로 Sepharose 2B를 이용한 2차 정제를 실시하여 최종적으로 균사체내 단백다당류의 탈이온수 분획물(PIIPDG)과 알칼리분획물(PIIPAG), 균사체외 단백다당류의 탈이온수 분획물(PIEPDG) 알칼리 분획물(PIEPAG)을 얻었다. 이때의 정제 수율은 1차 정제에서 40%의 회수율을 나타내었으며 2차 정제에서는 $38{\sim}61%$의 높은 회수율을 보였다. PIEPDG는 총당 79.0%, 총단백질 7.2%, PIEPAG는 총당 56.7%, 총단백질 40.8%, PIIPDG는 총당 64.8%, 총단백질 17.4%, PIIPAG는 총당 56.9%, 총단백질 41.5%으로 측정되었다. 각 단백다당류의 분자량은 PIEPDG 166KDa에서 PIEPAG 565KDa까지 모두 10만이 넘는 거대분자로 나타났다. 각 분획물의 단당류 조성을 볼때, PIEPDG는 glucose, PIIPDG와 PIIPAG는 glucose, inositol, PIEPAG는 glucose, rfructose, inositol이 검출되었다.

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송이균 배양을 위한 균사생장 조건 (Favorable Condition for Mycelial Growth of Tricholoma matsutake)

  • 김인엽;정광열;한상국;차주영;성재모
    • 한국균학회지
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    • 제33권1호
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    • pp.22-29
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    • 2005
  • 송이(Tricholoma matsutake)균을 고체배양과 액체배양에서 균사 생장의 적합한 조건을 구명함으로 앞으로 송이균을 대량 배양하여 접종함으로 송이를 생산할 수 있는 가능성을 얻기 위하여 본 연구를 실시하였다. 송이균은 고체배지의 경우 HA, TMM 배지에서 생장이 양호하였으며, 액체배지의 경우 PDB, TMM 배지에서 균사의 생장이 우수하게 나타났다. 온도에서는 $25^{\circ}C$에서 균사의 생장이 가장 효과적이었다. 송이균이 잘 생장하는 탄소원은 다당류인 Dextrin이고 질소원은 Yeast extract와 Peptone이고 $Fe_{2}(SO_{4})_{3}{\cdot}H_{2}O$와 KCl이었다. 액체배양에서는 균사의 생장은 플라스크 배양에서 진탕배양에서 정치배양보다 $2{\sim}7$배 정도의 균사의 생장이 좋았으며, 100 ml 가장 양호하였다. 균사의 절편을 삼각플라스크에 $6{\sim}7$개 넣어서 배양하는 것이 양호하였으며 배양기간은 접종 후 4주에서부터 균사의 생장과 펠릿의 분화가 나타나기 시작하여 9주까지 활발하게 생장하였다. 대량배양에서 균사생장이 양호한 배지로는 감자추출배지이었으며 8리터 병에 200 ml 접종량을 넣고 8주간 배양하면 송이의 균사체량이 가장 많이 얻을 수 있었다.

Bioluminescent Determination of Lactose Secretion: A Measure of the In Vitro Performance of Mammary Acini from Lactating Rats

  • Choi, B.H.;Stewart, K.W.;Davis, S.R.;Myung, K.H.
    • Asian-Australasian Journal of Animal Sciences
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    • 제15권2호
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    • pp.274-278
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    • 2002
  • A culture system for lactating rat mammary acini was evaluated, where the primary indicator of performance was lactose secretion, measured by a sensitive bioluminescence assay. Lactose secretion was reduced by half (p<0.01) over the first 6 h of culture by overnight feed withdrawal (FW) from tissue donors but was sensitive to increased glucose concentration in the culture media (p<0.001) up to 30 mM. Lactose production of cells from fed donors over the first 6 h in culture in 30 mM glucose was 8.9 fmol/cell/h - a rate calculated to be about half that in vivo. No significant difference was shown in lactose secretion by cells from fed or FW rats over 6-24 h. Lactose secretion was 3.6 fmol/cell/h by cells from fed animals in 40 mM glucose concentration media over the 6-24 h culture period. Addition of insulin to the culture media had no effect on rates of lactose secretion while addition of prolactin and hydrocortisone, with or without insulin, significantly (p<0.001) decreased lactose production over both 0-6 h and 6-24 h culture periods. Lactose synthesis in vitro was significantly enhanced by aeration of the media during collagenase digestion of mammary tissue (p<0.05). No improvement in lactose secretion was effected by shaking of cells during culture, Matrigel coating of culture dishes or change in cell density over a range up to 2.5 million cells per ml.

Production of Bacterial Cellulose by Gluconacetobacter hansenii PJK Isolated from Rotten Apple

  • Park, Joong-Kon;Park, Youn-Hee;Jung, Jae-Yong
    • Biotechnology and Bioprocess Engineering:BBE
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    • 제8권2호
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    • pp.83-88
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    • 2003
  • A cellulose-producing strain isolated from rotten apples was identified as Gluconacetobacter hansenii based on its physiological properties and the 16S rDNA complete sequencing method, and specifically named Gluconacetobacter hansenii PJK. The amount of bacterial cellulose (BC) produced by G. hansenii PJK in a shaking incubator was 1.5 times higher than that produced in a static culture. The addition of ethanol to the medium during cultivation enhanced the productivity of bacterial cellulose, plus the supplementation of 1% ethanol into the culture medium made the produced BC aggregate into a big lump and thus protected the bacterial-cellulose-producing G. hansenii PJK cells in the shear stress field from being converted into non-cellulose-producing (Cel) mutants. Cells subcultured three times in a medium containing ethanol retained their ability to produce BC without any loss in the production yield.

재조합 효모를 이용한 endoinulinase의 생산 특성

  • 한지혜;이은미;윤영미;이현철;정봉우;채건상
    • 한국생물공학회:학술대회논문집
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    • 한국생물공학회 2000년도 춘계학술발표대회
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    • pp.478-481
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    • 2000
  • The INU2 gene encoding an endoinulinase of Aspergillus ficuum was expressed by the Kluyveromyces marxianus INU1 promoter in a SUC2-deleted Saccharomyces cerevisiae to produce the endoinulinase free of an exoinulinase and an extracellular invertase in the culture medium. When inulin was included in the medium, a recombinant yeast strain produced the sufficient amount of the enzyme to make a halo around its colony. An expression of endoinulinase was dependent on the culture temperature and shaking. The highest expression of endoinulinase was observed at $30^{\circ}C$, and 150rpm.

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Myriococcum albomyces에 있어서 Cellulase 유도생성에 관한 연구 (Studies on Cellulase Induction in Myriococcum albomyces)

  • 정동효
    • 한국식품과학회지
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    • 제3권1호
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    • pp.1-5
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    • 1971
  • 1. 5% 밀기울 기본배지에다 inducer로서 CMC 혹은 Avicel을 첨가하여 Myriococcum albomyces를 접종하여 진탕배양할 때의 cellulase 유도 생성을 검토하였다. 2. DEAE-Sephadex A-25 column chromatography 법으로 배양액에서 cellulase 활성이 다른 3개의 부분, fraction I, fraction II 와 fraction III를 분리하였다. 3. Inducer로서 CMC첨가의 경우는 CMCase가 강해지고 반대로 Avicel을 가한 경우는 Avicelase가 강하였다.

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오미자의 형질전환된 근으로부터 리그난 화합물의 검출 (Detection of Lignans from Transformed Root Cultures of Schisandra chinensis Baillon)

  • 황성진;표병식;황백
    • 한국약용작물학회지
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    • 제12권6호
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    • pp.448-453
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    • 2004
  • Transformed roots of Schisandra chinensis were obtained following co-cultivation of in vitro cultivated plantlet segments with Agrobaterium rhizogens ATCC15834. This root was examined for its growth and gomisin J contents under various culture conditions. Among the six basal culture media tested, WPM (Lloyd & McCown, 1980) medium supplemented with 5% sucrose was the best roots growth 6.2 (g D.W/flask) and gomisin J accumulation 1.56 $(X10^{-3}\;ug/g\;D.W)$. Initial inoculum size correlated with the yield of biomass while gomisin J contents was not affect. Gomisin J production was influenced by the initial sucrose concentration and the highest production yield was achieved at the concentration of 7%. The optimal shaking speeds for roots growth and gomisin J production was 120 and 140 rpm, respectively.

수종 유황환원균주의 분리, 동정 및 그의 생리적 특성에 대하여 (Isolation Identification and Physiological Characteristics of Some Sulfur-Reducing Microbes)

  • 이민재;오명수
    • 미생물학회지
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    • 제10권4호
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    • pp.175-190
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    • 1972
  • This work was designed to illustrate physiological effects on the elimination of sulfur and its compounds in petroleum using sulfur-reducing bacteria. Deulfurizing bacteria were collected from sewage and soil at several areas in Soul and Ulsan, Korea. Seven supecies of sulfur-reducing microbes isolated were identified as : Pseudomonas marginata, Ps.effusa, Ps. putrefaciens, Ps.pseudcmcnelli, Ps. xanthochlora, Ps.bowlesiae, and Ps.aeruginosa. And some experiments were performed to define the growing characteristics of the Pseudomonads and the results obtained are as follows : 1) Shaking culture method was more effective for the growth of the cells than stagnant culture. 2) Beef peptone medium was better for the growth than other media. 3) Cuprous chloride of 50 ppm and cupper sulfate of 300 ppm treated, respectively, in the medium were effective for the growth. 4) Benzene of toluene of 5,000 ppm and petroleum ether of 50,000 ppm did not show remarkable inhibitory effects on the growth.

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벼 도열병균, pyricularia oryzae의 원형질체 형성 (Formation of protoplasts from pyricularia oryzae)

  • 이용환;정후섭
    • 미생물학회지
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    • 제23권3호
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    • pp.209-214
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    • 1985
  • The optimum conditions of protoplasts formation from Pyricularia oryzae were investigated with lytic enzymes and osmotic stabilizers. The mycelia were begun to refease the protoplasts in response to the complex enzyme solution after 30-60 minutes and reached to maximum after 2-3hrs. Among the lytic enzymes tested, the mixture solution containing ${\beta}-Glucuronidase$(0.01 ml/ml), Cellulase ONOZUKA-RS(20mg/ml), Driselase (10mg/ml), and Macerozyme R-10 (10mg/ml) resulted in the highest rate of protoplasts releasing of Pyricularia oryzae. The best stabilizer was 0.6M KCl at pH 7.0. Shen the mycelia were digested with enzyme mixture, the stationary culture was better than shaking culture for higher protoplast formation.

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The Bioconversion of Red Ginseng Ethanol Extract into Compound K by Saccharomyces cerevisiae HJ-014

  • Choi, Hak Joo;Kim, Eun A;Kim, Dong Hee;Shin, Kwang-Soo
    • Mycobiology
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    • 제42권3호
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    • pp.256-261
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    • 2014
  • A ${\beta}$-glucosidase producing yeast strain was isolated from Korean traditional rice wine. Based on the sequence of the YCL008c gene and analysis of the fatty acid composition, the isolate was identified as Saccharomyces cerevisiae strain HJ-014. S. cerevisiae HJ-014 produced ginsenoside Rd, $F_2$, and compound K from the ethanol extract of red ginseng. The production was increased by shaking culture, where the bioconversion efficiency was increased 2-fold compared to standing culture. The production of ginsenoside $F_2$ and compound K was time-dependent and thought to proceed by the transformation pathway of: red ginseng extract ${\rightarrow}Rd{\rightarrow}F_2{\rightarrow}$ compound K. The optimum incubation time and concentration of red ginseng extract for the production of compound K was 96 hr and 4.5% (w/v), respectively.