• KSBB Journal
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• 제11권3호
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• pp.311-316
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• 1996

Polyethylene glycolCPEG)의 재조합 효모 배양 에서의 세포성장과 glucoamylase 생산에 대한 영향에 대하여 조사하였다. PEG 첨가에 의하여 세포성 장은 영향을 받지 않았으나 재조합 glucoamylase의 생산은 증가되었다. 최척의 PEG 분자량은 6000이었으며 최척의 농도는 1g/L이었다. 이러한 최척의 값을 이용하여 PEG 첨가배지에서 첨가하지 않은 배지보다 약 23%의 세포외 glucoamylase 활성의 증가를 보였다.

• Journal of Microbiology and Biotechnology
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• 제11권1호
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• pp.13-16
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• 2001

Maltose and soluble starch were used as secondary sources of carbon for glucoamylase production by Aspergillus awamori in solid state fermentation. During batch cultivation, maltose above 2.5%(w/w) repressed glucoamylase production, but, by adding either 2.5% (w/w) maltose or 1.25% (w/w) soluble starch to fed-batch cultivations, glucoamylase activity was increased by 15% and 170% over standard medium, respectively. The data showed that maltose is a weak inducer of glucoamylase production in solid stat fermentation.

• 한국미생물·생명공학회지
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• 제16권6호
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• pp.494-498
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• 1988

Starch로부터 직접적으로 ethanol을 발효 생산할 수 있는 새로운 효모균주의 개발을 목적으로 S. diastaticus의 glucoamylase gene을 cloning vector를 사용하지 않고 S. cerevisiae에 transformation시켜, soluble starch를 직접 발효 할 수 있는 transformants를 얻는데 성공하였으며 이들 중 glucoamylase 생성능이 가장 우수한 균주인 TSD-14를 전보에서 선별하였다. Transformant TSD-14의 glucoamylase 생성조건과 ethanol productivity를 parent strain과 비교 검토한 결과 이들 성질에 있어서 TSD-14는 donor인 S. diastaticus와 거의 유사하였다. 즉, 탄소원으로는 soluble starch가 균의 생육 및 효소생성에 가장 효과적이었으며 glucose, maltose 등은 균의 생육에는 효과적이었으나 효소생성은 저해하였다. 질소원으로 무기태 질소원에 비하여 유기태 질소원이 좋은 효과를 나타냈으며 특히, peptone과 yeast extract가 효과적이었다. 또한 금속염으로는 FeSO$_4$, MgSO$_4$, MnCl$_2$, NiSO$_4$등이 효과적이었으며 CoCl$_2$, HgCl$_2$, PbCl$_2$등은 오히려 균의 생육뿐만 아니라 효소생성을 크게 저해하였다. 한편, TSD-14의 ethanol productivity를 조사한 결과, 15% sucrose, soluble starch, liquefied potato starch 등에서 8.3% (v/v) , 4.8%(v/v), 7.5%(v/v)의 ethanol을 생성하여 각각 총당에 대해 84%, 45%, 70%의 발효율을 나타냈다.

• 한국미생물·생명공학회지
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• 제17권5호
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• pp.519-523
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• 1989

Aspergillus sp.로부터 glucoamylase를 생성키 위한 조건을 검토하였다. 곰팡이는 탄소원으로 soluble starch, 질소원으로 yeast extract를 사용했을 때 최대 효소생성을 얻을 수 있었다. 그리고, 탄소원 및 질소원의 농도에 따른 효소생성은 soluble starch를 5%, yeast extract를 1% 수준으로 사용했을 때 효소생성은 극대화하였다. 또한 배지의 초기 pH를 6.0, 그리고 배양온도를 28$^{\circ}C$로 유지했을 때 효소생성이 높았다. 고체배지를 사용했을 때에는, 밀기울 배지가 glucoamylase 생성을 위해서 가장 효과가 좋았다.

• Journal of Microbiology and Biotechnology
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• 제25권2호
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• pp.185-195
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• 2015

Glucoamylase is an important industrial enzyme. Glucoamylase production by industrial Aspergillus niger strain featured with two major problems: (i) empirical substrate feeding methods deteriorating the fermentation performance; and (ii) the high raw materials cost limiting the economics of the glucoamylase product with delegated specification. In this study, we first proposed a novel three-stage varied-rate substrate feeding strategy for efficient glucoamylase production in a 5 L bioreactor using the standard feeding medium, by comparing the changing patterns of the important physiological parameters such as DO, OUR, RQ, etc., when using different substrate feeding strategies. With this strategy, the glucoamylase activity and productivity reached higher levels of 11,000 U/ml and 84.6 U/ml/h, respectively. The performance enhancement in this case was beneficial from the following results: DO and OUR could be controlled at the higher levels (30%, 43.83 mmol/l/h), while RQ was maintained at a stable/lower level of 0.60 simultaneously throughout the fed-batch phase. Based on this three-stage varied-rate substrate feeding strategy, we further evaluated the economics of using alternative carbon sources, attempting to reduce the raw materials cost. The results revealed that cornstarch hydrolysate could be considered as the best carbon source to replace the standard and expensive feeding medium. In this case, the production cost of the glucoamylase with delegated specification (5,000 U/ml) could be saved by more than 61% while the product quality be ensured simultaneously. The proposed strategy showed application potential in improving the economics of industrial glucoamylase production.

• 한국식품영양과학회지
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• 제14권2호
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• pp.188-191
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• 1985

퇴비 숙성초기에 고온성 cellulose 분해이용균으로 분리된 Herpetosiphon geysericola CUM 317균주는 전분분해 효소인 ${\alpha}-amylase,\;{\beta}-amylase$ 및 glucoamylase를 모두 생성한다. 이 균을 사용하여 그 배양조건을 달리하여 각 amylase의 생성관계를 서로 비교한바 50℃의 밀기울 고체배지나 $40^{\circ}C$의 액체배지상에서 ${\beta}-amylase$는 배양초기 10시간만에 최대의 생성력가를 보였는 반면, ${\alpha}-amylase$와 glucoamylase는 30 내지 40시간 정도의 배양말기에 최대를 이루었다. Polypeptone을 함유한 액체배지에 탄소원의 첨가나 무기질소원의 첨가는 전반적으로 amylase들의 생성이 크게 저하되었으나 cellulose에 의해서 glucoamylase의 경우 150% 정도 증가되었다. 액체배지에 $CuSO_4$를 첨가해 줌으로서 ${\alpha}-amylase$만의 생성증가 효과를 얻었고 $CdSO_4$에 의하여 ${\beta}-amylase$만의 생성증가가 있었으며, 그리고 $CaCl_2$에 의하여 glucoamylase만의 증가효과가 있은 반면, 상대적으로 ${\beta}-amylase$의 급격한 감소가 일어났다. 이들 amylase들의 최적 효소생성 pH는 7.5였으며, 최적온도는 ${\alpha}-amylase$와 glucoamylase의 경우 $40^{\circ}C$였고 ${\beta}-amylase$는 $30^{\circ}C$였다.

• 미생물학회지
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• 제14권2호
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• pp.49-49
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• 1976

Enzyme activities, such as glucoamylase dextrinogenic amylase, cellulase, acid protase and neutral protease, of Rhizopus isolated from various substrates collected throughout South Korea are measured, and their enzyme activities are surveyed from taxonomical, ecological and physiological viewpoint. Effect of carbon sources and phytohormones on the amylalse production of Rhizopus are also measured. Among the 735 strains of Phizopus isolated, strain number 587 exhibiting most prominent dextrinogenic amylase and netral protease activity is selected as the best strain, and the strain number 673, 108, 329, 165 and 728 are seleted for their predominant cellulase, acid protease, glucoamylase, dextrinogenic amylase and neutral protease activities, respectively. R.acidus and R.nigricans which exhibited relatively higher callulalse activity, showed lower activities for both amylase. R.tritici exhibited higher protease activity. The relations between activities and various substrates of wild strains are not outstnading difference, although the strains isolated from inland region exhibited more or less higher amylase and cellulase activities, than those of coast region, generally. Lactose and dextrin are most effective carbon sources for glucoamylase and dextrinogenic amylase production of the Rhizopus niveus, respectively. Although all phytohormones tested are effective for production of amylase by the Rhizopus strains, except nicotinamide for glucoamylase production, biotin and ascorbate are most effective for dextrinogenic amylase and glucoamylase production, respectively.

• 미생물학회지
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• 제14권2호
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• pp.47-56
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• 1976

Enzyme activities, such as glucoamylase dextrinogenic amylase, cellulase, acid protase and neutral protease, of Rhizopus isolated from various substrates collected throughout South Korea are measured, and their enzyme activities are surveyed from taxonomical, ecological and physiological viewpoint. Effect of carbon sources and phytohormones on the amylalse production of Rhizopus are also measured. Among the 735 strains of Phizopus isolated, strain number 587 exhibiting most prominent dextrinogenic amylase and netral protease activity is selected as the best strain, and the strain number 673, 108, 329, 165 and 728 are seleted for their predominant cellulase, acid protease, glucoamylase, dextrinogenic amylase and neutral protease activities, respectively. R.acidus and R.nigricans which exhibited relatively higher callulalse activity, showed lower activities for both amylase. R.tritici exhibited higher protease activity. The relations between activities and various substrates of wild strains are not outstnading difference, although the strains isolated from inland region exhibited more or less higher amylase and cellulase activities, than those of coast region, generally. Lactose and dextrin are most effective carbon sources for glucoamylase and dextrinogenic amylase production of the Rhizopus niveus, respectively. Although all phytohormones tested are effective for production of amylase by the Rhizopus strains, except nicotinamide for glucoamylase production, biotin and ascorbate are most effective for dextrinogenic amylase and glucoamylase production, respectively.

• 한국식품과학회지
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• 제32권4호
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• pp.875-880
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• 2000

Cryptococcus laurentii Y-23의 glucoamylase와 exopolygalacturonase(exo-PGase)의 생산에서 당류성 유도기질들과 무기염들이 미치는 영향을 조사하였다. 당류들에 의한 영향을 조사한 결과, soluble starch와 dextrin은 높은 glucoamylase의 생산만을 유도하였으나 pectin은 exo-PGase와 glucoamylase의 생산을 함께 유도하였으며, glucose는 glucoamylase의 생산을 유도하지 못하였으나 pectic acid는 약간의 exo-PGase의 생산을 유도하였다. 발효조에서 5일간 배양하면서 유도기질들에 의한 효소생산성 등을 조사한 결과, 균은 대략 배양 12시간경부터 대수기가 시작되어 대부분 36시간경에 정상기에 도달하였다. Glucoamylase의 생산성은 배지에 soluble starch만 첨가하였을 때 배양 72-86 시간경에 가장 높았고, exo-PGase의 생산성은 pectin만 첨가하는 것 보다 pectin과 soluble starch를 동시첨가 하였을 때 더 높았으며, 또한 배지에 ammonium sulfate가 존재하지 않을 경우 배양 pH가 계속 증가되어 두 효소의 생산성이 현저히 감소하였다. 무기염에 의한 영향을 조사한 결과, $Mn^{2+}$은 무첨가 대조구에 비하여 glucoamylase와 exo-PGase의 생산성을 각각 21%와 18%씩 증가시켰다.

• 미생물학회지
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• 제18권4호
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• pp.161-171
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• 1980

A mutant strain having increased productivity of both enzymes, protease and amylase, was obtained from A. flavus KU 153, isolatd from South Korea for its high protease production by successive ultra-violet light irradiation, Two glucoamylases from the mutant strain selected were purified from wheat branculture by successive salting out, followed by dialysis and column chromatography, and their characteristics were compared with those of the wild strain. Glucoamylase production of the mutant selected was increased about 3.3 times compared with the wild strain, and 2.1 times compared with the parental strain, ${\alpha}-amylase$ activity of the mutant selected was about 2 times hugher than that of the wild strain or the parental strain. Protease and cellulase productivities of the muant selected were all alike compared with those of the highly proteolytic mutant, the parental strain. Therefore, it was considered that the back mutation on the protease production did not occurred in the formation process of the glucoamylase producing mutant. Total activities of glucoamylase I and II from the mutant selected were 2.86 and 3.65 times higher compared with those from the wild strain, respectively. Considering the optimal pH-thermal stability and Km-Vmax value of glucoamylase I and II from both strains, wild and mutant, it was deduced that the characteristics of glucoamylase I and II from the wild strain did not altered during the mutation process. Therefore, it was concluded that the selected mutant did not induce the formation of another glucoamylase isozyme, or the changes in the characteristics of the glucoamylase, but induce the productivity of the same glucoamylase I and II by the action of regulatory gene.