• 한국식품과학회지
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• 제20권3호
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• pp.344-349
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• 1988

분획(分劃)된 대두(大豆) 7S 및 11S 단백질(蛋白質)은 단백가수분해(蛋白加水分解) 효소(酵素)(alcalase 및 pronase)로 1시간(時間)동안 가수분해(加水分解)하였을 때 사용(使用)된 효소(酵素) 및 단백질(蛋白質) 종류(種類)에 관계없이 pH 5에서 용해도(溶解度), 열응고성(熱凝固性) 및 $Ca^{++}$에 대한 내침전성(耐沈殿性)은 상당히 증가(增加)에멀젼 활성 및 거품 안정성(安定性)은 감소(減少), 에멀젼 열안정성(熱安定性) 및 동점도(動粘度)는 거의 변화(變化)되지 않았다. 그러나 용해도(溶解度)에서 7S 단백질(蛋白質)은 pH 6에서 11S 단백질(蛋白質)은 pH 4에서 감소(減少)하였으며 또한 11S 단백질(蛋白質)은 유흡수성(油吸收性) 및 거품 형함능(形咸能)에서 가수분해(加水分解)에 의하여 증가(增加)하였으나 7S 단백질(蛋白質)은 거의 변화(變化)하지 않았다.

• Molecules and Cells
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• 제41권11호
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• pp.933-942
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• 2018

Traditionally, small-molecule or antibody-based therapies against human diseases have been designed to inhibit the enzymatic activity or compete for the ligand binding sites of pathological target proteins. Despite its demonstrated effectiveness, such as in cancer treatment, this approach is often limited by recurring drug resistance. More importantly, not all molecular targets are enzymes or receptors with druggable 'hot spots' that can be directly occupied by active site-directed inhibitors. Recently, a promising new paradigm has been created, in which small-molecule chemicals harness the naturally occurring protein quality control machinery of the ubiquitin-proteasome system to specifically eradicate disease-causing proteins in cells. Such 'chemically induced protein degradation' may provide unprecedented opportunities for targeting proteins that are inherently undruggable, such as structural scaffolds and other non-enzymatic molecules, for therapeutic purposes. This review focuses on surveying recent progress in developing E3-guided proteolysis-targeting chimeras (PROTACs) and small-molecule chemical modulators of deubiquitinating enzymes upstream of or on the proteasome.

• Asian-Australasian Journal of Animal Sciences
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• 제33권1호
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• pp.100-110
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• 2020

Objective: The objective of this study was to isolate proteolytic microorganisms and evaluate their effects on proteolysis in total mixed ration (TMR) silages of soybean curd residue. Methods: TMRs were formulated with soybean curd residue, alfalfa or Leymus chinensis hay, corn meal, soybean meal, a vitamin-mineral supplement, and salt in a ratio of 25.0: 40.0:30.0:4.0:0.5:0.5, respectively, on a basis of dry matter. The microbial proteinases during ensiling were characterized, the dominate strains associated with proteolysis were identified, and their enzymatic characterization were evaluated in alfalfa (A-TMR) and Leymus chinensis (L-TMR) TMR silages containing soybean curd residue. Results: Both A-TMR and L-TMR silages were well preserved, with low pH and high lactic acid concentrations. The aerobic bacteria and yeast counts in both TMR silages decreased to about 10⁵ cfu/g fresh matter (FM) and below the detection limit, respectively. The lactic acid bacteria count increased to 10⁹ cfu/g FM. The total microbial proteinases activities reached their maximums during the early ensiling stage and then reduced in both TMR silages with fermentation prolonged. Metalloproteinase was the main proteinase when the total proteinases activities reached their maximums, and when ensiling terminated, metallo and serine proteinases played equally important parts in proteolysis in both TMR silages. Strains in the genera Curtobacterium and Paenibacillus were identified as the most dominant proteolytic bacteria in A-TMR and L-TMR, respectively, and both their proteinases were mainly with metalloproteinase characteristics. In the latter ensiling phase, Enterococcus faecium strains became the major sources of proteolytic enzymes in both TMR silages. Their proteinases were mainly of metallo and serine proteinases classes in this experiment. Conclusion: Proteolytic aerobic bacteria were substituted by proteolytic lactic acid bacteria during ensiling, and the microbial serine and metallo proteinases in these strains played leading roles in proteolysis in TMR silages.

• Bulletin of the Korean Chemical Society
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• 제11권6호
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• pp.534-538
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• 1990

Glucagon was found to interact with DMPC vesicles electrostatically and hydrophobically. It appears that glucagon bound irreversibly to the vesicles through hydrophobic interaction was partially protected from the proteolysis by trypsin. Out of three possible sites, only the peptide bond preceded by Arg-18 was cleaved by a prolonged trypsin treatment. ${\alpha}$-chymotrysin did not affect the vesicle-bound glucagon. Based on these observations, possible structure of irreversibly bound glucagon on the vesicle surface is discussed.

• 약학회지
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• 제38권2호
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• pp.202-210
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• 1994

To investigate the feasibility of mucosal delivery of $[D-Ala^6]$ LHRH, a potent analogue of LHRH, enzymatic proteolysis of $[D-Ala^6]$ LHRH and inhibitory effect of medium chain fatty acid salts(MFA) were studied using rabbit mucosal homogenate. $[D-Ala^6]$ LHRH incubated in homogenates of rectal(RE), nasal(NA) and vaginal(VA) mucosa were assayed by HPLC. The degradation of $[D-Ala^6]$ LHRH followed the first order kinetics. The degradation products were found as $[D-Ala^6]$ $LHRH^{1-7}$(m-i), to a lesser extent, $[D-Ala^6]$ $LHRH^{1-9}$(m-ii) and $[D-Ala^6]$ $LHRH^{1-3}$(m-iii) by the method of amino acid analysis(PITC method). The formation of$[D-Ala^6]$ $LHRH^{1-7}$ was not inhibited by the addition of disodium ethylenediaminetetraacetic acid but inhibited by sodium tauro-24,25-dihydrofusidate, suggesting that endopeptidase 24.11(EP 24.11) cleaves the $Leu^7-Arg^8$ bond of $[D-Ala^6]$ LHRH and is the primary $[D-Ala^6]$ LHRH degrading enzyme. The patterns of $[D-Ala^6]$ LHRH degradation indicated that EP 24.11 exists in each mucosal homogenate with the order of RE>NA>VA. MFA significantly inhibited the proteolysis of $[D-Ala^6]$ LHRH. The addition of sodium caprate(1.0%) or sodium laurate(0.5%) to the each mucosal homogenate completely protected $[D-Ala^6]$ LHRH from the degradation.

• 한국식품조리과학회지
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• 제13권2호
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• pp.168-172
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• 1997

체내 소화효소에 대한 안정성을 검토하기 위해 competitive ELISA를 이용하여 항원 결합력의 변화를 조사하였다. YIgG는 펩신에 대해 상당히 불안정하여 pH 2.0에서 30분간의 반응에 의해 항원 결합력이 소실되었다. 한편 yIgG 용액에 50%(w/v) saccharose를 첨가하여 펩신과 30분 반응시킨 결과 native yIgG에 비해 항원 결합력이 6.7배 정도 저하되었으나 미첨가시에 비해 항원 결합력이 상당히 유지되었으므로, 펩신에 대한 yIgG의 안정성은 saccharose에 의해 상당히 증가되었음을 알 수 있다. YIgG는 트립신 및 키모트립신과 반응 후 항원 결합력의 큰 저하는 나타나지 않아 펩신에 비해 상당히 안정한 것으로 생각된다. 트립신과 8시간 반응 후 yIgG의 항원 결합력은 native yIgG에 비해 2배 감소되었으나 키모트립신과 8시간 반응 후 yIgG의 항원 결합력은 1.5배 감소되었다. 그러므로 yIgG는 키모트립신 대해 가장 안정하였다.

• 약학회지
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• 제51권3호
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• pp.199-205
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• 2007

Thermostable asparaginase was purified to homogeneity from mesophilic Strepfomyces lincolnensis M-20 by 30${\sim}$70% ammonium sulfate precipitation and asparagine-Sepharose CL 6B affinity column chromatography, The apparent molecular mass of L-asparaginase by SDS-PAGE was found to be 47 kDa, whereas by its mobility on Sephacryl S-300 column was around 180 kDa, indicating that the enzyme at the native stage acts as tetramer, The purified enzyme showed a single band on acrylamide gel electrophoresis. The optimum pH and temperature were pH 9.5 and 55${\circ}$C, respectively. Chemical modification experiments of purified asparagines implied the existence cystein residue located at or near active site. Purified asparaginase retained the 85% of the initial activity after incubation at 90${\circ}$C for 30 min. A correlation between themostability and resistance to proteolysis of commercial asparaginase and purified asparaginase from Strepfomyces lincolnensis M-20 was investigated. Purified thermostable asparaginase was resistant to trypsin and chymotrypsin treatment, while the commercial asparaginase was not themostable and was susceptible to proteolytic treatment with trypsin and chymotrypsin.

• Journal of Microbiology and Biotechnology
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• 제9권5호
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• pp.679-682
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• 1999

When the human parathyroid hormone (hPTH) is expressed as a secretory product in S. cerevisiae, most of the secreted hPTH is internally cleaved by endoproteolytic processing. To investigate whether the yeast endoproteases such as Kex2p, Yap3p, and Mkc7p are involved in the endoproteolytic processing of hPTH in S. cerevisiae, hPTH was expressed in S. cerevisiae mutants deficient in one or two of the following well-known endoproteases such as Kex2p, Mkc7p, and Yap3p. Among these mutants, the yap3-disrupted(yap3$\Delta$) and yap3/mkc7-disrupted (yap3Δmkc7$\Delta$) yeasts showed a significant reduction in the extent of hPTH proteolysis. In contrast, the mkc7-disrupted (mkc7$\Delta$) yeast did not reduce the proteolysis of hPTH as compared to the wild type. This suggests that Mkc7p is not involved in the endoproteolytic processing of hPTH. It was also found that the kex2-disrupted (kex2$\Delta$) mutant was not able to secrete a detectable amount of hPTH.

• Food Science and Biotechnology
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• 제14권3호
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• pp.355-357
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• 2005

This study evaluated the binding abilities of rabbit anti-ovalbumin (OVA) immunoglobulin G (IgG) and egg-allergic patient IgE on gamma-irradiated OVA during proteolysis using pepsin and trypsin. The concentrations of both the intact and the irradiated OVAs decreased during proteolysis when detected with IgG However, when detected by patient IgE the concentration of the intact OVA decreased up to 30 min after the trypsin treatment and increased thereafter. Irradiated OVA detected by patient IgE showed a lower initial concentration (0.16%) than that of the intact OVA, and this reduced concentration was maintained stably. The results indicate that irradiation, rather than enzymatic treatment, could reduce the binding of the irradiated and enzyme-treated OVA. Therefore, gamma irradiation has potential as an effective method to reduce OVA-induced allergy and may enhance the safety of egg-allergic individuals.

• 한국작물학회지
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• 제38권4호
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• pp.350-359
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• 1993

수도 여절편의 단백질함량 감소는 KCI처리에 의해 촉진된다. 본 연구는 KCI이 증가 시키는 단백질 분해작용을 더욱 촉진시키기 위한 시도의 하나로 GA$_3$와 ABA를 KCI과 혼합처리한 다음, 이들이 노화엽의 단백질 분해작용을 조절하는 기작을 구명하기 위하여 수행하였다. 파종후 16～18일된 실행의 제2본엽을 5cm 길이로 잘라 test 용액에 배양하는 8일간 단백질, aminotks, 흡수량, 단백질 분해효소의 활성과 단백질 분해산물인 aminotks의 유출량 변화 드을 조사하였다. 1. GA$_3$ 단독처리는 잎의 단백질 감소에 큰 영향을 미치지 않았고, KCI과 혼합처리되어도 KCI 단독처리와 비교할 때 유의적인 변화를 유기하지 않았다. 그러나 ABA 단독처리는 단백질분해, amino산의 유출 및 endoproteinase 활성을 현저히 증가시켰고, ABA와 KCI의 혼합처리는 이들의 증가에 상조적이었다. 2. KCI은 Rubisco를 분해하는 exoproteinases의 활성을 감소시키는데 반해 GA$_3$나 ABA 첨가는 모두 이의 감소를 완화시키는 효과가 있었다. 그러나 KCI이 처리된 잎의 endoproteinase 활성은 ABA와의 혼합처리에 의해서만 상조적인 증가를 나타내어 이러한 효과가 없는 GA$_3$와는 그 기능이 대조적이었다. 3. 배양기간중 잎의 흡수량이 낮을수록 단백질 감소량이 많고 그 속도도 빨랐다. ABA와 KCI의 혼합처리로 단백질이 가장 많이 감소하였던 잎의 흡수량이 가장 낮아, 단백질 분해작용과 흡수률 사이에 깊은 관련이 있음을 시사하였다. 4. 따라서 KCI에 의한 수도 엽절편의 단백질분해촉진은 endoproteinases 활성과 감소 등에 그 원인이 있고, ABA는 이러한 변화에 상조적으로 작용하나 GA$_3$는 큰 영향이 없음을 알 수 있었다.다.e 및 free fatty acid) 는 13.3～17.4%로 나타났다.로 빠른 시일에 집중적인 연구가 필요하다고 본다.다. 4. 저온저장(4$^{\circ}C$, RH 50%)한 벼는 2년반 저장한 벼도 밥맛의 변화가 거의 없었다. 5. 1988년산 및 1989년산 일반계를 10분도와 12분도로 도정하였을 때 도정도에 따른 밥맛의 차이는 없었다.X>$CoO_x$는 $Co_3O_4$로 존재하고, 반응 전의 경우에는 이와는 다른 chemical state를 보여주었다. XRD 및 XPS 결과를 바탕으로, 촉매표면에 존재하는 $Co_3O_4$의 외부표면이 $Co_2TiO_4$와 $CoTiO_3$ 같은 $CoTiO_x$로 encapsulation되어 있는 모델구조를 제안할 수 있고, 이는 반응시간의 함수로 나타나는 촉매활성에 있어서 전이영역의 존재를 잘 설명할 수 있을 뿐만 아니라, XRD와 XPS에서 얻어진 촉매의 물리화학적인 특성을 잘 반영할 수 있다. 나타냈고, 골격근과 눈 조직에서 피루브산에 대한 LDH의 친화력이 상당히 크므로 LDH가 혐기적 조건에서 효율적으로 기능을 하는 것으로 사료된다.5) and "Cleanliness of clothes ＆ features" (p ＜0.05) of VIP ward were significantly higher than those of a general ward.tive to apply.아울러 고려(考慮)해야 한다. 이것은 고무기술자(技術者)가 당면(當面)해야할 과제(課題)에 속(屬)하며 바람직 한것은 본장(本章)의 내용(內容)이 여러 상황하(狀況下)에서 당면(當面)한 문제(問題)에 대(對)해 어떻게 대처(對處)해 야 할지를 모르는 여러 기술자(技術者)들에게 도움이 되었으면 하는 것이다. 얻어짐을 알았다. 여기서의 합성분말을