• 대한생식의학회:학술대회논문집
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• 2001.06a
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• pp.76.2-77
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• 2001

• Proceedings of the Zoological Society Korea Conference
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• 1997.10b
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• pp.310.1-310
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• 1997

• KSBB Journal
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• v.7 no.4
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• pp.284-289
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• 1992

The optimum conditions for the production of tryptophan using a recombinant Klebsiella pnuemoniae phe A tyr A trp R/pSC 101-$trp^{+}$ and its plasmid stability during tryptophan production were studied. The optimum temperature was $37^{\circ}C$ and the specific growth rate was 1.05$h^{-1}$ at $37^{\circ}C$. Tryptophan production was increased by glucose fed-batch culture, and tryptophan was accumulated to 0.175 g/l after 36 hrs. This amount was about 1.2 and 1.6 times greater than that obtained from batch culture and flask culture, respectively. The stability of the strain in fed-batch cu1ture was greatly different from that in repeated flask culture. After 6 generation, 95% of total cells was stable in repeated flash culture, but in fed-batch culture only 50% was stable.

• Applied Biological Chemistry
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• v.40 no.1
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• pp.18-22
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• 1997

The conditions for production of high cell density of Bifidobacterium longum were investigated and the cross-flow filtration system was used to remove the inhibitory metabolites, lactic acid and acetic acid. The maximum cell growth was observed with glucose as carbon source at the concentration of 50 g/l at $37^{\circ}C$ with the initial pH 6.5. When B. longum was cultured in a cross-flow filtration system, the maximum cell growth was observed at a dilution rate(D) of $0.31\;h^{-1}$ and the dry cell weight was 16.4 g/l($3.5{\times}10^{10}\;cell/ml$), which was about four times higher than that obtained in the batch culture with pH control.

• Korean Journal of Plant Tissue Culture
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• v.25 no.4
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• pp.263-266
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• 1998

Flowergenic callus was induced from the ovary surface of Allium fistulosum L. cultured on MS medium containing 0.5mg/L NAA and 0.5mg/L BA or 0.5mg/L kinetin. After 3-4 weeks of culture, the flower buds were developed from flowergenic callus. The continuous production of flowergenic callus was proliferated, when subcultured on the medium containing 0.5mg/L NAA and 0.5mg/L kinetin. However, frequency of flower bud formation from flowergenic callus was decreased as the subculture was repeated. Histological observation reveals that the developmental pattern of flower bud from flowergenic callus was closely similar to that of natural flowers.

• The Science & Technology
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• v.32 no.7 s.362
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• pp.78-79
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• 1999

유전공학기법으로 산삼이나 가시오갈피 등 약재를 대량 생산할 수 있는 새로운 기술을 개발하고 있는 (주)마이크로프랜츠는 주목받는 벤처기업이다. 전주에 있는 이 기업은 생약제재의 종자에서 분리한 세포를 액체 배지에서 배양한 다음 증식된 세포들을 체세포배 발생 과정을 거친 결과 뿌리와 잎을 갖춘 유식물체(싹이 튼 식물체)를 얻는데 성공했다. 이러한 조직배양 방법은 완전 무공해 약재를 생산할 수 있고 6년 걸리는 자연재배를 3개월이며 생산할 수 있는 장점을 지니고 있다.

• Proceedings of the Korean Society of Developmental Biology Conference
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• 2001.02a
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• pp.68-70
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• 2001

착상전 초기배아에서 용해된 Matrigedl에 의한 배아의 형태발생, 세포증식, apoptosis 및 UPK활성의 변화를 조사하였다. Matrigel (0.5%)을 첨가한 배양액에서 체외배양된 2-세포기 배아의 형태발생 및 포배당 세포수가 증가되었으며 (GF>GFR>control) 포배의 TUNEL 양성 할구 및 배아내 caspase-3의 활성이 감소되었다. (GF

• Proceedings of the Korean Society for Applied Microbiology Conference
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• 1976.04a
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• pp.182.4-182
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• 1976

음이온계 합성세제인 ABS(alkyl benzene sulfonate)의 분해능이 우수한 균주를 자연계에서 분리하여 Pseudomonas caryophylli로 동정하였다. ABS 10 ppm을 함유한 인공폐수에서 분리 균주를 배양시 ABS는 40％이상, BOD는 89％, COD는 71％ 감소되었으며 ABS분해능은 자연미생물군에 의한 혼합배양시의 2배이상이었다. 분리균주에 의한 시판합성세제의 분해율은 Hlti 46.2％, Kleenup 37.5％, No. 1 39％, OK 37.8％이었다.

• Korean Chemical Engineering Research
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• v.47 no.2
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• pp.220-229
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• 2009

Strain improvement and morphology investigation in bioreactor cultures were undertaken in suspended cultures of Phellinus linteus mycelia for mass production of protein-bound polysaccharides(soluble ${\beta}$-D-glucan), a powerful immuno-stimulating agent. Phellineus sp. screened for this research was identified as Phellinus linteues through ITS rDNA sequencing method and blast search, demonstrating 99.7% similarity to other Phellinus linteus strains. Intensive strain improvement program was carried out by obtaining large amounts of protoplasts for the isolation of single cell colonies. Rapid and large screening of high-yielding producers was possible because large numbers of protoplasts ($1{\times}10^5{\sim}10^6\;protoplasts/ml$) formed using the banding filtration method with the cell wall-disrupting enzymes could be regenerated in relatively high regeneration frequency($10^{-2}{\sim}10^{-3}$) in the newly developed regeneration medium. It was demonstrated that the strains showing high performances in the protoplast regeneration and solid growth medium were able to produce 5.8~6.4%(w/w) of ${\beta}$-D-glucan and 13~15 g/L of biomass in stable manners in suspended shake-flask cultures of P. linteus mycelia. In addition, cell mass increase was observed to be the most important in order to enhance ${\beta}$-D-glucan productivity during the course of strain improvement program, since the amount of ${\beta}$-D-glucan extracted from the cell wall of P. linteus mycelia was almost constant on the unit biomass basis. Therefore we fully investigated the fungal cell morphology, generally known as one of the key factors affecting cell growth extent in the bioreactor cultures of mycelial fungal cells. It was found that, in order to obtain as high cell mass as possible in the final production bioreactor cultures, the producing cells should be proliferated in condensed filamentous forms in the growth cultures, and optimum amounts of these filamentous cells should be transferred as active inoculums to the production bioreactor. In this case, ideal morphologies consisting of compacted pellets less than 0.5mm in diameter were successfully induced in the production cultures, resulting in shorter period of lag phase, 1.5 fold higher specific cell growth rate and 3.3 fold increase in the final biomass production as compared to the parallel bioreactor cultures of different morphological forms. It was concluded that not only the high-yielding but also the good morphological characteristics led to the significantly higher biomass production and ${\beta}$-D-glucan productivity in the final production cultures.

• Korean Journal of Plant Tissue Culture
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• v.28 no.6
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• pp.335-339
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• 2001

Grapevine leafroll-associated 3 closterovirus (GLRaV-3) is phloem limited virus, and one of the most severe viral diseases found in Korea. However, nonhomogenous distribution and low concentration and seasonal variations of GLRaV-3 in grapevines remain as main problems which prevent the introduction and molecular biology or serology experiments. Virus-infected plantlet in vitro was obtained from node tissue cuttings, which was GLRaV-3 infected 'kyoho' vines. The amount of purified virus was highest in vitro plantlet. Moreover, viruses seem to be relatively homogeneously distributed in all organs including leaf, stem and callus derived from in vitro plantlets. RT-PCR detection using in vitro plantlet tissue as template was most effective. When comparing ELISA to RT-PCR, RT-PCR detection was 1,000 times as effective as ELISA. These results can be explained by improved quality such as tenderness or less tannins in plantlet in vitro. In conclusion, until infected herbaceous host will be available, tissue culture can be usefully adopted as a technique for a good source of GLRaV-3 closterovirus for further studies.