• 제목/요약/키워드: bovine serum albumin (BSA)

검색결과 307건 처리시간 0.021초

국내산 무화과에서 추출한 protease 조효소액의 안정성과 최적화에 관한 연구 (Stabilizing and Optimizing Properties of Crude Protease Extracted from Korean Figs)

  • 김미현;노정해;김미정
    • 한국식품조리과학회지
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    • 제27권3호
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    • pp.29-37
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    • 2011
  • 국내산 무화과(Ficus carica L.) 중의 조효소를 추출하고 단백분해 조효소의 활성도를 측정하였다. 무화과를 균질화하여 원심분리한 조효소액은 41.15 mM/g fig의 활성을 나타내었으며 단백질 침전 후 조효소액은 17.65 mM/g fig의 활성을 나타내었다. 무화과 조효소액의 기질 특이성은 casein > egg white > BSA > myofibrilar protein > collagen > elastin 등의 순이었다. 무화과 단백질 분해 조효소의 안정성을 보면 pH 6.5~9.0에서 안정하며 pH 2~3의 강산에서는 실활하였다. 또한 $60^{\circ}C$까지는 역가의 변화가 거의 없으며 그 이상의 온도에서는 급격히 활성의 감소를 보이고 있다. 염에 대해서는 0.7 M 정도의 소금 농도에서까지는 비교적 안정하나 그 이후로는 안정성이 떨어지는 것으로 나타났다. 조효소활성에 대한 pH의 영향을 보면 pH 7~8에서 높은 활성을 나타냈으며 근원섬유에 대한 단백 분해능이 pH에 매우 민감한 것으로 나타났다. 무화과 단백질 분해 조효소의 활성은 $40^{\circ}C$ 이후부터 조효소의 활성이 증가하기 시작하여 $60^{\circ}C$에서 최적 활성을 나타내었고 그 이상의 온도에서 점차적으로 다시 감소하였다. $80^{\circ}C$에서도 근원섬유에 대한 단백 분해활성은 최고치에 비해 50% 정도에 해당하는 것으로써 무화과 조효소가 비교적 온도에 민감하지 않았다. 또한 염 농도는 최적 활성에 큰 영향을 미치지 않았다. 무화과를 사용한 sauce 등을 제조할 때에 이러한 특성들을 이해한다면 우리나라 육류 요리용의 우수한 연육제품을 제조할 수 있을 것이다.

Comparative Studies of Protein Modification Mediated by Fenton-like Reactions of Iron, Hematin, and Hemoglobin: Generation of Different Reactive Oxidizing Species

  • Kim, Young-Myeong;Kim, Sung-Soo;Kang, Gu;Yoo, Yeong-Min;Kim, Ki-Mo;Lee, Mi-Eun;Han, Jeong-A;Hong, Sun-Joo
    • BMB Reports
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    • 제31권2호
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    • pp.161-169
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    • 1998
  • TThe reactive oxygen species oxidatively modify the biological macromolecules, including proteins, lipids, and nucleic acids. Iron- and heme-mediated Fenton-like reactions produce different pro-oxidants. However, these reactive products have not been clearly characterized. We examined the nature of the oxidizing species from the different iron sources by measuring oxidative protein modification and spectroscopic study. Hemoglobin (Hb) and methemoglobin (metHb) were oxidatively modified in $O{\array-\\\dot{2}}$ and $H_{2}O_{2}$ generating systems. Globin and bovine serum albumin (BSA) were also modified by iron, iron-EDTA, hematin, and Hb in an $O{\array-\\\dot{2}}$ generating system. In a $H_{2}O_{2}$ generating system, the iron- and iron-EDTA-mediated protein modifications were markedly reduced while the Hb-and hematin-mediated modifications were slightly increased. In the $O{\array-\\\dot{2}}$ generating system, the iron- and iron-EDTA-mediated protein modifications were strongly inhibited by superoxide dismutase (SOD) or catalase, but heme- and Hb-mediated protein modifications were inhibited only by catalase and slightly increased by SOD. Mannitol, 5,5-dimethyl-l-pyrroline-N-oxide (DMPO), deoxyribose, and thiourea inhibited the iron-EDTA-mediated protein modification. Mannitol and DMPO, however, did not exhibit significant inhibition in the hematin-mediated modification. Desferrioxamine (DFO) inhibited protein modification mediated by iron, but cyanide and azide did not, while the hematin-mediated protein modification was inhibited by cyanide and azide, but not significantly by DFO. The protein-modified products by iron and heme were different. ESR and UV-visible spectroscopy detected the DMPO spin adduct of the hydroxyl radical and ferryl ion generated from iron-EDTA and metHb, respectively. These results led us to conclude that the main oxidizing species are hydroxyl radical in the iron-EDTA type and the ferry I ion in the hematin type, the latter being more effective for protein modification.

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유지방구로부터 분리한 Lipase의 활성에 미치는 pH의 영향 (Effects of pH on the Activity of Lipase Isolated from Milk Fat Globules)

  • 김거유
    • 한국축산식품학회지
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    • 제20권2호
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    • pp.101-106
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    • 2000
  • 유지방구로부터 분리 정제한 lipase의 활성과 안정성에 미치는 pH의 영향을 야자유와 균질유를 기질로 하여 조사하였다. 효소원으로 buttermilk를 사용하였을 경우는 반응온도 $37^{\circ}C$에서 야자유, 균질유 모두 pH 9.5에서 최대 활성을 나타내었으며, 전형적인 종형의 pH의 존곡선을 나타내었다. 그러나 반응온도 $0^{\circ}C$에서는 pH 10.0까지 활성이 증가하였다. 정제 lipase를 사용한 경우는 반응응도 $37^{\circ}C$에서 균질유를 기질로 사용하였을 때 종 모양의 곡선을 나타내었으며, 최대 활성은 pH 9.0에서 나타났다. 반응온도 $0^{\circ}C$에서는 pH 10.0까지 활성이 계속 증가하였다. BSA를 첨가한 야자유를 기질로 사용한 경우는 반응온도 $37^{\circ}C$, $0^{\circ}C$ 모두 최대 활성이 pH 9.5에 나타났으며, pH 10.0에서는 활성이 현저하게 저하하였다. 정제 lipase의 안정성에 미치는 pH의 증가에 따라 현저하게 저하하였다. pH 10.0에서 $37^{\circ}C$로 20분간 효소를 유지하였을 경우 lipase의 활성은 pH 8.5 때의 활성에 비하여 13%로 감소하였다. 그러나, $4^{\circ}C$에서 60분간 효소를 유지하였을 경우는 lipase 활성이 pH 7.5∼10.0의 범위에서 안정하였다.

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한국산 메밀, 수수, 기장, 율무의 항산화효과 및 돌연변이억제효과 (Antioxidative and Antimutagenic Effects of Korean Buckwheat, Sorghum, Millet and Job기s Tears)

  • 곽충실;임수진;김성애;박상철;이미숙
    • 한국식품영양과학회지
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    • 제33권6호
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    • pp.921-929
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    • 2004
  • 한국산 메밀, 수수, 기장, 율무의 돌연변이억제효과와 항산화효과 및 총 flavonoid와 polyphenol 함량을 측정하였다. 이를 위하여 에탄을 추출시료를 얻은 후 Ames test 방법으로 돌연변이 억제효과를 검색하였고, Fe$^{2+}$로 유도된 지질과산화 억제율, DPPH 라디 칼 소거율 및 MDA-BSA 결합억제율을 측정하는 3가지 방법으로 항산화효과를 검정하고, 총 flavonoid와 polyphenol 함량을 측정한 결과를 요약하면 다음과 같다. 에탄올 추출시료의 $IC_{50}$/에 의한 지질과산화 억제효과를 비교한 결과 메밀(0.174 mg/ assay), 수수(0.241 mg/assay), 율무(1.891 mg/assay), 기장(2.873 mg/assay) 순이었으며 에탄을 추출시료의 $IC_{50}$/을 계산하여 DPPH 라디칼 제거능을 비교한 결과 메밀(0.264 mg/assay), 수수(2.135 mg/assay), 기장(2.902 mg/assay), 율무(4.667 mg/assay) 순이었다. 지질과산화물-단백질 결합 억제효과는 에탄을 추출시료의 $IC_{50}$/을 기준으로 비교한 결과 메밀(3.73 mg/assay), 율무(51.82 mg/assay), 기장(120.59 mg/assay), 수수(449.43mg/assay)의 순이었다. S. Typhimurium TA98에서 에탄올 추출물 4.5 mg/assay농도에서 2-Nitrofluorene에 의 한 직접돌연변이를 저해하는 비율은 수수(50.2%), 기장(20.3%), 메밀(18.5%), 율무(17.5%)의 순이었으며, S. Typhimurium TA100에서 sodium azide에 의한 직접돌연변이를 저해하는 비율은 기장(100%), 율무(78.6%), 수수(23.7%), 메밀(10.1%)의 순이었다. S. Typhimurium TA98 또는 TA100에서 에탄올 추출물이 2-Anthramine에 의한 간접돌연변이 억제효과는 기장, 수수, 율무, 메밀 모두 우수하였으며, 특히 기장과 수수의 효과가 매우 좋았다. 총 flavonoid 함량은 메밀(1.41mg/g), 수수(1.17 mg/g), 기장(0.96 mg/g), 율무(0.66 mg/g)순이었고, 총 polyphenol 함량은 메밀(3.71 mg/g), 수수(1.76 mg/g), 율무(1.7 mg/g), 기장(1.09 mg/g) 순으로 각각 DPPH 라디칼제거효과 및 지질과산화억제효과의 순과 일치하였다. 총 flavonoid 함량은 DPPH 라디칼 제거효과에 대한 $IC_{50}$/ 값과 높은 상관관계(r=-0.9924, p<0.01)를 나타내었다.

Dibutyryl Cyclic AMP가 생쥐여포난자의 성숙에 미치는 억제효과에 관한 자기방사법적 연구 (Autoradiographic Studies on the Inhibitory Effect of Dibutyryl Cyclic AMP on Mouse Oocyte Maturation in Vitro)

  • 최춘근
    • Applied Microscopy
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    • 제7권1호
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    • pp.21-43
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    • 1977
  • This experiment was undertaken in order to localize the labeled dbcAMP (dibutyryl cyclic AMP) in oocytes whose development has been suppressed by cold dbcAMP for 6 or 19 hours in vitro. Mouse oocytes were obtained from the ovaries of 3-4 week old A strain female mice, by puncturing the Graafian follicles in the modified Krebs-Ringer bicarbonate salt solution under the dissecting microscope. Those oocytes which have intact germinal vesicle were cultured in the basic culture medium supplemented with 0.4% bovine serum albumin (BSA). Cultivation of the oocytes was carried out in a microtube developed by Cho (1974). The cultures were then incubated in a humidified 5% $CO_2$ incubator maintained at $37^{\circ}C$ for 6 or 19 hours (Donahue, 1968). DbcAMP was added to culture medium for a final concentration of 100ug/ml, and $^3H-dbc$ AMP (specific activity 13 Ci/mM) for a final concentration of $40{\mu}Ci/ml$ was also added to the medium. For electron microscopic autoradiography, those oocytes recovered from the culture were washed with phosphate buffer (pH 7.4), and immediately prefixed in a 2.5% glutaraldehyde overnight and postfixed for 2 hours at $4 ^{\circ}C$ in 1% osmium tetroxide in phosphate buffer with pH 7.4 (Palade, 1952). After fixation, the materials were dehydrated in graded alcohol series and embedded in Epon 812 mixture based on the standard procedures (Luft, 1961). The thin sections $600-700{\AA}$ thick were mounted on the grids of 200 meshes. The grids containing sections were coated with a nuclear emulsion Kodak NTB-3 and stored in a cold dark box (at $4^{\circ}C$) for 3 weeks. After exposure, the samples were developed with Kodak D-19 and stained with uranyl acetate and lead citrate. Routine observation was made with Hitachi HU-11E electron microsocope. The results of the observation were as followings: 1. It was found that the labeled dbcAMP penetrated the egg plasma membrane and dispersed at random in the cytoplasm. 2. It was also observed that most of the labeled dbcAMP was attached to microfibrillar lattices portion of the oocyte cytoplasm. There fore, it is presumed that the receptor of the dbcAMP is localized in the microfibrillar lattices of the oocyte. 3. It also seems that some other cell organells such as mitochondria, Golgi complex, cortical granules are not directly related to the action of the dbcAMP. 4. The labeled dbcAMP was neither observed in the membrane nor in the nucleus. Therefore, it seems that there is no relationship between the concentration of dbcAMP and the nuclear membranous permeability. 5. There was no difference in number of dbcAMP particles when oocytes were cultured for 6 hours and 19 hours. 6. However, it was observed that, in same of the oocytes suppressed in germinal vesicle by dbcAMP for 19 hours, cell organells were moved and concentrated to a small portion of the cytoplasm, and that the morphology of the organells greatly changed to an abnormal. form. Therefore, it is supposed that those oocytes were in the process of degeneration. From the above results, it is expected that dbcAMP penetrated the egg membrane and was bound to the receptor which seems to be located in the microfibrillar lattiees portion, and that this dbcAMP-receptor complex inhibited some enzyme system of the oocytes which are essential for the germinal vesicle breakdown.

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체외배양에서 인간 난포액이 생쥐의 배 발달에 미치는 영향 (The Effects of Human Follicular Fluid on Embryonal Development of Mouse in In Vitro Culture)

  • 민부기;최기욱;김기석;이희섭;홍기연;이봉주;이선영;박승택
    • Clinical and Experimental Reproductive Medicine
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    • 제26권2호
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    • pp.171-178
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    • 1999
  • The follicular fluid (FF) of ovary contains various biological active products which affected on the growth of follicles and the fertilization of oocyte in physiological reproductive process of mammals. This study was designed to determine the effects of human FF on fertilization of oocyte and embryonal development in vitro culture. The FF was prepared as clear without blood contamination by needle aspiration from mature follicles of human at the time of oocytes retrieval for in vitro fertilization (IVF). As the medium for culture in vitro of embryonal cells, human tubal fluid (HTF) supplemented with follicular fluids at concentrations of 10%, 40% and pure FF were used. These effects were compared to control group of cultured embryos in HTF supplemented with 0.4% BSA (bovine serum albumin). For IVF, 64 eggs in control group, 67 eggs in 10% FF, 57 eggs in 40% FF and 64 eggs in pure FF were respectively allocated. And the rates of fertilization were almost similar in all groups as resulting 82.81% in control, 85.07% in 10% FF, 87.71% in 40% FF and 81.25% in pure FF. On the examination for embryonal cleavage from fertilized eggs, the rates of developing to 4 cell stage was similar in all groups, as results 98.11% in control, 98.27% in 10% FF and 98% in 40% FF but 78.84% in pure FF. And the rates of developing to 8-16 cell stage were significantly reduced as 44% in 40% FF and 44.23% in pure FF (p<0.05) compare to 71.69% in control media. As likewise, the rates of developing to morular stage were also significantly reduced to 36% (p<0.05) and 21.15% (p<0.01) respectively in 40% FF and pure FF. And the rates to blastocystic stage of embryo was lowest as 7.69% in pure FF (Table 1). The quality of embryonal cells on cleavage to the 8-16 cell stage was poorer, higher concentrations of FF. The rates of grade 1 in pure FF, as 23.07%, was lowest compare to those of other groups, in which the rates of grade 1 in control, 10% FF and 40% FF were 58.49%, 47.36% and 34% respectively. And on the contrary, the rate of grade 4 in pure FF was highest as 23.07%, while those were 5.66% in control, 8.77% in 10% FF and 20% in 40% FF (Table 2). On the viability of embryos, the rate of embryonal cell death was more rise, at the higher concentrations as well as longer exposure in the follicular fluid. At 48 hours after in vitro culture of embryos, the rate of survival embryos in pure FF was markedly lowered as 44.23%, compare to that of control (p<0.05). But there was not significant difference between the rates of survival embryos in each group beside the pure FF, which the rates were 77.35% in control, 70.17% in 10% FF and 60% in 40% FF respectively. And at 72 hours after in vitro culture, the rates of survival embryos were also significantly dropped to 21.15% in pure and 36% in 40% at concentration of FF compare to 62.26% in control (p<0.05, p<0.01). Finally, the rate of embryonal death at 96 hours after in vitro culture was highest as 82.69% in pure FF among all groups which those were 35.84 in control, 56.14% in 10% FF and 64% in 40% FF respectively (Fig. 1, 2, 3). In conclusion, this study suggests that the FF has no effects, in particular, to the in vitro fertilization of oocytes but exerted a bad effect to the cleavage, quality and viability of the embryonal cells during in vitro culture. However, the FF is harmful on embryonal development at conditions in higher concentration and especially on the embryos after $8{\sim}16$ cell stage.

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착상 전 유전진단 기술 개발의 동물실험 모델로서 할구 생검된 생쥐 배아에서 동결보존 융해 후 배아 발생 양상과 공배양 효과에 관한 연구 (Developmental competence and Effects of Coculture after Crypreservation of Blastomere-Biopsied Mouse Embryos as a Preclinical Model for Preimplantation Genetic Diagnosis)

  • 김석현;김희선;류범용;최성미;방명걸;오선경;지병철;서창석;최영민;김정구;문신용;이진용;채희동;김정훈
    • Clinical and Experimental Reproductive Medicine
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    • 제27권1호
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    • pp.47-57
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    • 2000
  • Objective: The effects of cryopreservation with or without coculture on the in vitro development of blastomere-biopsied 8-cell mouse embryos were investigated. This experimental study was originally designed for the setup of a preclinical mouse model for the preimplantation genetic diagnosis (PGD) in human. Methods: Eight-cell embryos were obtained after in vitro fertilization (IVF) from F1 hybrid mice (C57BL(표현불가)/CBA(표현불가)). Using micromanipulation, one to four blastomeres were aspirated through a hole made in the zona pellucida by zona drilling (ZD) with acid Tyrode's solution (ATS). A slow-freezing and rapid-thawing protocol with 1.5M dimethyl sulfoxide (DMSO) and 0.1M sucrose as cryoprotectant was used for the cryopreservation of blastomere- biopsied 8-cell mouse embryos. After thawing, embryos were cultured for 110 hours in Ham's F-10 supplemented with 0.4% bovine serum albumin (BSA). In the coculture group, embryos were cultured for 110 hours on the monolayer of Vero cells in the same medium. The blastocyst formation was recorded, and the embryos developed beyond blastocyst stage were stained with 10% Giemsa to count the total number of nuclei in each embryo. Results: The survival rate of embryos after cryopreservation was significantly lower in the blastomere-biopsied (7/8, 6/8, 5/8, and 4/8 embryos) groups than in the non-biopsied, zona intact (ZI) group. Without the coculture, the blastocyst formation rate of embryos after cryopreservation was not significantly different among ZI, the zona drilling only (ZD), and the balstomere-biopsied groups, but it was significantly lower than in the non-cryopreserved control group. The mean number of cells in embryos beyond blastocyst stage was significantly higher in the control group ($50.2{\pm}14.0$) than in 6/8 ($26.5{\pm}6.2$), 5/8 ($25.0{\pm}5.5$), and 4/8 ($17.8{\pm}7.8$) groups. With the coculture using Vero cells, the blastocyst formation rate of embryos after cryopreservation was significantly lower in 5/8 and 4/8 groups, compared with the control, 7/8, and 6/8 groups. The mean number of cells in embryos beyond blastocyst stage was also significantly lower in 4/8 group ($25.9{\pm}10.2$), compared with the control ($50.2{\pm}14.0$), 7/8 ($56.0{\pm}22.2$), and 6/8 ($55.3{\pm}25.5$) groups. Conclusion: After cryopreservation, blastomere-biopsied mouse embryos have a significantly impaired developmental competence in vitro, but this detrimental effect might be prevented by the coculture with Vero cells in 8-cell mouse embryos biopsied one or two blastomeres. Biopsy of mouse embryos after ZD with ATS is a safe and highly efficient preclinical model for PGD of human embryos.

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