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1.
Purification and characterization of trypsin from the spleen of tongol tuna (Thunnus tonggol) 总被引:1,自引:0,他引:1
Klomklao S Benjakul S Visessanguan W Kishimura H Simpson BK 《Journal of agricultural and food chemistry》2006,54(15):5617-5622
Trypsin from tongol tuna (Thunnus tonggol) spleen was purified to 402-fold by ammonium sulfate precipitation, followed by a series of chromatographic separations. The molecular mass of trypsin was estimated to be 24 kDa by size-exclusion chromatography and sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE). Trypsin appearing as a single band on native PAGE showed the maximal activity at pH 8.5 and 65 degrees C. It was stable in a wide pH range of 6-11 but unstable at the temperatures greater than 50 degrees C. The enzyme required calcium ion for thermal stability. The activity was strongly inhibited by 1.0 g/L soybean trypsin inhibitor and 5 mM TLCK and partially inhibited by 2 mM ethylenediaminetetraacetic acid. Activity was lowered with an increasing NaCl concentration (0-30%). The enzyme had a Km for Nalpha-p-tosyl-L-arginine methyl ester hydrochloride of 0.25 mM and a Kcat of 200 s-1. The N-terminal amino acid sequence of trypsin was determined as IVGGYECQAHSQPHQVSLNA and was very homologous to other trypsins. 相似文献
2.
Chen YT Hsu LH Huang IP Tsai TC Lee GC Shaw JF 《Journal of agricultural and food chemistry》2007,55(3):714-722
A chitinase cDNA clone (CpCHI, 1002 bp) was isolated from papaya fruit, which encoded a 275 amino acid protein containing a 28 amino acid signal peptide in the N-terminal end. The predicted molecular mass of the mature protein was 26.2 kDa, and its pI value was 6.32. On the basis of its amino acid sequence homology with other plant chitinases, it was classified as a class IV chitinase. An active recombinant CpCHI enzyme was overexpressed in Escherichia coli. The purified recombinant papaya chitinase showed an optimal reaction temperature at 30 degrees C and a broad optimal pH ranging from 5.0 to 9.0. The recombinant enzyme was quite stable, retaining >64% activity for 3 weeks at 30 degrees C. The spore germination of Alternaria brassicicola could be completely inhibited by a 76 nM level of recombinant CpCHI. Recombinant CpCHI also showed antibacterial activity in which 50% of E. coli was inhibited by a 2.5 microM concentration of the enzyme. 相似文献
3.
U Luzzana T Mentasti J Opstvedt E Nyg?rd V M Moretti F Valfrè 《Journal of agricultural and food chemistry》1999,47(7):2879-2884
The racemization kinetics of aspartic acid in heat-treated whole herring have been studied under conditions of treatment comparable to those that may occur in processing of fish meal. D-Aspartic acid content in the samples has been measured by RP-HPLC with precolumn automatic derivatization. The major parameters affecting the rate of racemization of aspartic acid k(Asp) have been demonstrated to be temperature (elevation of temperature from 95 to 120 degrees C resulted in an increase of k(Asp) from 0.46 to 3.39x10(-3) min(-1)), moisture of the raw material (reduction of the moisture content of the raw material from 80 to 15% lowered k(Asp) measured at 95 degrees C from 0.46 to 0.06x10(-3) min(-1)), and to a lesser extent, pH (k(Asp) at 95 degrees C was lowered from 0.46 to 0.37x10(-3) min(-1) following a decrease of pH from 7.0 to 4.0). No significant effects on the racemization rate of aspartic acid was observed for reducing the oxygen pressure to 0.8%. The results from the present study show that the content of D-aspartic acid in fish material is a function of heat exposure and may be used to predict the thermal history of fish meal. 相似文献
4.
This study was carried out to investigate the enzymatic hydrolysis conditions on the properties of protein hydrolysate from fish muscle of the marine fish species Collichthys niveatus. About 160 fish samples were tested, and the analyzed fish species was found to be a lean fish with low fat (1.77 ± 0.01%) and high protein (16.76 ± 1.21%). Fish muscle of C. niveatus was carefully collected and hydrolyzed with four commercial enzymes: Alcalase, Neutrase, Protamex, and Flavourzyme under the conditions recommended by the manufacturers. Among the tested proteases, Neutrase catalyzed the hydrolysis process most effectively since the hydrolysate generated by Neutrase has the highest content of sweet and umami taste amino acids (SUA). The effect of hydrolysis conditions was further optimized using response surface methodology (RSM), and the optimum values for temperature, pH, and enzyme/substrate ratio (E/S ratio) were found to be 40.7 °C, 7.68, and 0.84%, respectively. Finally, the amino acid composition of the hydrolysate was analyzed by AccQ·Tag derivatization and HPLC-PDA determination. Major amino acids of the muscle of C. niveatus were threonine, glutamic acid, phenyalanine, tryptophan, and lysine, accounting for respectively 10.92%, 10.85%, 10.79%, 9.86%, and 9.76% of total amino acid content. The total content of essential amino acids was 970.7 ng·mL(-1), while that of nonessential amino acids was 709.1 ng·mL(-1). The results suggest that the fish muscle and its protein hydrolysate from C. niveatus provide a versatile supply of the benefits and can be incorporated as supplements in health-care foods. 相似文献
5.
为了制备风味良好的鲣鱼调味基料,本试验以鲣鱼蒸煮液(STCL)为原料,在酶解和脱腥基础上,采用感官评价、电子鼻技术结合主成分分析(PCA)及线性判别分析(LDA),通过正交试验优化美拉德工艺,并对鲣鱼蒸煮液酶解液美拉德产物进行氨基酸组成成分分析和必需氨基酸营养评价。结果表明,电子鼻技术结合LDA优于PCA,更能客观地区分不同条件下鲣鱼蒸煮液酶解液美拉德反应产物的风味差异;鲣鱼蒸煮液酶解液美拉德反应最优工艺条件为:添加木糖-葡萄糖1:2,在110℃下加热45 min,在此条件下,美拉德产物鱼香味浓郁,色泽呈黄棕色,氨基酸总量为7.036 g·100g-1,必需氨基酸含量为2.888 g·100g-1,必需氨基酸指数(EAAI)为64.034,说明鲣鱼蒸者液美拉德反应产物营养价值较高,是研发海鲜调味料的理想基料。本研究结果为鲣鱼调味基料的开发提供了一定的理论依据。 相似文献
6.
Medina I Satué-Gracia MT German JB Frankel EN 《Journal of agricultural and food chemistry》1999,47(12):4873-4879
Polyphenols extracted from extra virgin olive oil (EVOO) were tested for their ability to inhibit lipid oxidation of canned tuna. Hydroperoxide formation during oxidation was monitored by measurement of peroxide value and decomposition of hydroperoxides by static headspace gas chromatographic analysis of volatiles. In tuna oxidized at 40 and 100 degrees C, 400 ppm of the EVOO polyphenols was an effective antioxidant as compared with 100 ppm of a 1:1 mixture of the synthetic antioxidants butylated hydroxytoluene and butylated hydroxyanisole. However, at concentrations <100 ppm, the EVOO phenolic compounds promoted hydroperoxide formation and decomposition. The EVOO polyphenols were effective antioxidants when added to heated tuna muscle in the presence of either brine or refined olive oil. The oxidation rate in tuna muscle packed in brine was higher than that of tuna packed in refined olive oil. The EVOO polyphenols had higher antioxidant activity in the brine samples than in the refined olive oil. The higher antioxidant activity of EVOO polyphenols in tuna packed in brine may be explained by their greater affinity toward the more polar interface between water and the fish oil system. 相似文献
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草鱼leptin基因的分离鉴定及在巴斯德毕赤酵母中的表达 总被引:1,自引:0,他引:1
利用RT-PCR技术扩增出草鱼(Ctenopharyngodonidellus)的leptin基因,将leptin基因克隆至真核表达载体pPIC9K,电穿孔转化GS115菌株,经G418筛选和甲醇诱导后,对表达产物进行SDS-PAGE琼脂糖凝胶电泳和Westernblot分析。结果表明,草鱼leptin基因cDNA序列由438个核苷酸组成,编码146个氨基酸组成的多肽(GenBank登陆号AY551335),与鲤鱼(Cyprinuscarpio)leptin基因相比,核苷酸和氨基酸的同源性为99%;与人、猪和鼠相比,核苷酸同源性分别为84%、86%和95%,氯基酸的同源性分别为84%、82%和96%;与河豚(Takifugurubripes)相比,氨基酸具有较大的差异,仅有9%的同源性,表明leptin在物种的进化上具有一定的差异;实现了草鱼leptin基因在毕赤酵母(Pichiapastoris)中的表达,表达蛋白的分子量约为16kD,Westernblot分析表明,表达产物具有一定的免疫学活性。 相似文献
10.
为分析不同复合保鲜膜处理对金枪鱼的保鲜效果,以鱼鳞明胶为主料,添加桔子/柠檬精油和薄荷制备可食性保鲜膜,用于金枪鱼肉的冷藏保鲜,检测冷藏过程中金枪鱼肉的TVB-N值、pH值、菌落总数、肌红蛋白与高铁肌红蛋白含量、a*值、TBA值的变化,并对金枪鱼的品质进行感官评价分析。结果表明,鱼鳞明胶膜中添加薄荷、桔子精油和柠檬精油均能不同程度地抑制金枪鱼肉中的微生物繁殖,减缓TVB-N值、TBA值和高铁肌红蛋白含量的升高,抑制鱼肉色泽的衰变,且薄荷与桔子/柠檬精油的复合有协同增效保鲜金枪鱼肉的作用。明胶膜中复合2%浓度的桔子/柠檬精油对金枪鱼肉风味略有覆盖,低浓度桔子/柠檬精油(1%)有优化金枪鱼鱼肉气味的作用,且以柠檬精油的效果更优,1%薄荷-1%桔子精油-鱼鳞明胶复合膜和1%薄荷-1%柠檬精油-鱼鳞明胶复合膜保鲜处理的金枪鱼肉的货架期可分别延长至 7 d 和8 d。本研究结果为制备高品质水产品可食性保鲜膜材料提供了理论依据和技术支持。 相似文献
11.
Hu JM Li H Cao LX Wu PC Zhang CT Sang SL Zhang XY Chen MJ Lu JQ Liu YH 《Journal of agricultural and food chemistry》2007,55(6):2217-2224
The gene bgaP encoding cold-active beta-galactosidase from a psychrotrophic and halotolerant Planococcus sp. L4 was cloned into Escherichia coli and sequenced. A sequence analysis of the DNA responsible for the BgaP gene revealed an open reading frame of 2031 bp encoding for a protein of 677 amino acid residues. The BgaP was heterologously expressed in E. coli and purified followed by Ni2+ affinity chromatography. The molecular mass of the native enzyme was approximately 156 kDa as determined by gel filtration. The results of sodium dodecyl sulfate-polyacrylamide gel electrophoresis and the deduced amino acid sequence of the BgaP indicated molecular masses of 78 and 77.311 kDa, respectively, suggesting that the BgaP is a dimer. The purified BgaP had an isoelectric point of 4.8 and exhibited maximal activity at 20 degrees C and pH 6.8 under the assay conditions used. The enzyme is particularly thermolabile, losing all activity in only 10 min at 45 degrees C. It was able to hydrolyze lactose as a substrate, as well as o-nitrophenyl-beta-D-galactopyranoside (ONPG); the Km values with ONPG and lactose were calculated to be 5.4 and 20.4 mM at 5 degrees C, respectively. The catalytic efficiencies of BagP for lactose at 5 and 20 degrees C had 14 and 47 times more than that of E. coli beta-galactosidase at 20 degrees C, respectively. Therefore, cold-active beta-galactosidase from the psychrotrophic and halotolerant Planococcus sp. L4 could conceivably be developed to fulfill the practical requirements to enable its use for lactose removal in milk and dairy products at low temperature or a reporter enzyme for psychrophilic genetic systems. 相似文献
12.
M Ogawa S Nakamura Y Horimoto H An T Tsuchiya S Nakai 《Journal of agricultural and food chemistry》1999,47(8):3309-3318
Actomyosins (AMs) isolated from tilapia, lemon sole, ling cod, and rock fish were heated at 40 degrees C, and structural changes in AMs were investigated using Raman spectroscopy to elucidate low-temperature gelling phenomenon, that is, "setting", of surimi. The following conformational transitions were observed in lemon sole, ling cod, and rock fish gels during setting: a slow unfolding of alpha-helix and exposure of hydrophobic amino acid residues occurring in long-time incubation at 40 degrees C, thereby forming hydrophobic interactions among AM molecules. In addition, the most frequent conformation in disulfide bonds was gauche-gauche-trans (g-g-t) form in the set gel. On the other hand, tilapia AM did not form a gel with heating at 40 degrees C, its alpha-helical structure in the myosin being far more stable than that of the other species. The heat resistance of the tight alpha-helix may prevent the gelation of tilapia AM. It is, therefore, likely that the unfolding of the alpha-helix of myosin is a prerequisite for gelation of AM during setting. 相似文献
13.
Chaijan M Benjakul S Visessanguan W Lee S Faustman C 《Journal of agricultural and food chemistry》2007,55(11):4562-4568
The interaction between fish myoglobin (Mb) and natural actomyosin (NAM) extracted from fresh and frozen fish was studied. The quantity of soluble Mb in Mb-NAM extracted was less in frozen than in fresh fish (P < 0.05). However, no differences were observed in Mb that remained in solution following preparation of Mb-NAM from frozen whole fish vs frozen fillets (P > 0.05). MetMb formation in Mb-NAM was generally greater than that observed in control Mb (P < 0.05); the greatest MetMb content occurred in Mb-NAM extracted from frozen whole fish (P < 0.05). The effect of different aldehyde oxidation products on the interaction between fish Mb and NAM was also studied in vitro. The loss of soluble Mb from NAM:Mb preparations was greater in the presence of hexenal and hexanal (P < 0.05) relative to controls, and the degree of solubility loss varied with aldehyde type. Hexenal caused greater OxyMb oxidation than hexanal (P < 0.05). Whiteness of washed NAM and NAM-Mb mixtures decreased following aldehyde addition (P < 0.05). In the absence of Mb, the Ca2+ -ATPase activity of NAM was lower with added hexenal than with hexanal (P < 0.05). However, no differences in Ca2+ -ATPase activity between hexanal and hexenal-treated samples were observed when Mb was present (P > 0.05). Reducing and nonreducing sodium dodecyl sulfate-polyacrylamide gel electrophoresis analyses suggested that both disulfide and nondisulfide covalent linkages contributed to aldehyde-induced cross-linking between Mb and myofibrillar proteins. 相似文献
14.
R Barone R Briante S D'Auria F Febbraio C Vaccaro L Del Giudice G M Borrelli N Di Fonzo R Nucci 《Journal of agricultural and food chemistry》1999,47(5):1924-1931
Purification of a lipoxygenase enzyme from the cultivar Tresor of durum wheat semolina (Triticum turgidum var. durum Desf) was reinvestigated furnishing a new procedure. The 895-fold purified homogeneous enzyme showed a monomeric structure with a molecular mass of 95 +/- 5 kDa. Among the substrates tested, linoleic acid showed the highest k(cat)/K(m) value; a beta-carotene bleaching activity was also detected. The enzyme optimal activity was at pH 6. 8 on linoleic acid as substrate and at pH 5.2 for the bleaching activity on beta-carotene, both assayed at 25 degrees C. The dependence of lipoxygenase activity on temperature showed a maximum at 40 degrees C for linoleic acid and at 60 degrees C for bleaching activity on beta-carotene. The amino acid composition showed the presence of only one tryptophan residue per monomer. Far-UV circular dichroism studies carried out at 25 degrees C in acidic, neutral, and basic regions revealed that the protein possesses a secondary structure content with a high percentage of alpha- and beta-structures. Near-UV circular dichroism, at 25 degrees C and at the same pH values, pointed out a strong perturbation of the tertiary structure in the acidic and basic regions compared to the neutral pH condition. Moreover, far-UV CD spectra studying the effects of the temperature on alpha-helix content revealed that the melting point of the alpha-helix is at 60 degrees C at pH 5.0, whereas it was at 50 degrees C at pH 6.8 and 9.0. The NH(2)-terminal sequence allowed a homology comparison with other lipoxygenase sequences from mammalian and vegetable sources. 相似文献
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Michael J.W. Stokesbury John D. Neilson Edward Susko Steven J. Cooke 《Biological conservation》2011,144(11):2684-2691
The abundance of Atlantic bluefin tuna has been severely reduced since the advent of industrial fishing. A recreational catch-and-release fishery is currently being developed to target bluefin tuna in the southern Gulf of St. Lawrence, off the coast of Prince Edward Island, Canada. To evaluate the sustainability of this fishery, it is necessary to quantify post-release mortality for use in management models. Using pop-up archival satellite tags, we estimated the post-release mortality rate of bluefin tuna captured and released in an experimental recreational fishery. Fish were captured using bait on circle hooks and all fish were hooked in the jaw. Fish were released without being brought onboard the boat. Tags reported from 2 to 246 days post release. Two of 59 bluefin tuna died after catch-and-release yielding a mortality rate of 3.4% (95% C.I. = 0.8% < u < 12.6%). Four tags failed to report. Alternate estimates of the rate or mortality that included an incidental mortality (5.1%; 95% C.I. = 1.6% < u < 14.4%) and removal of the four tags that did not report from the sample (5.6%; 95% C.I. = 1.8% < u < 15.6%) were calculated. The range of fight times was 6–79 min (mean of 33 min; SD of 21 min). These data provide the first mortality estimates for angled and released bluefin tuna and will enable managers to evaluate the potential for developing a catch-and-release fishery in the southern Gulf of St. Lawrence. 相似文献
17.
Orlien V Risbo J Andersen ML Skibsted LH 《Journal of agricultural and food chemistry》2003,51(1):211-217
The thermal behavior of fresh tuna muscle, rehydrated freeze-dried tuna muscle, and tuna sarcoplasmic protein fraction was studied by three types of differential scanning calorimetry (DSC): conventional DSC, alternating DSC, and sensitive micro-DSC. The relationship between glass transition temperature, T(g), and water content was established. Only a low-temperature glass transition was detected for fresh tuna and freeze-dried tuna rehydrated to high water contents, whereas for sarcoplasmic protein fraction both a low-temperature and an apparent high-temperature glass transition were detected for samples of high water content. Construction of the supplemented state diagrams for whole tuna muscle and for tuna sarcoplasmic protein fraction confirmed the low-temperature transition to be glass transition of the maximally freeze-dehydrated phase. The apparent upper transition of sarcoplasmic protein fraction was shown not to be a glass transition but rather to originate from the onset of melting of ice, and the temperature of this event should be denoted T(m)'. The glass transition temperature and the concentration of the maximally freeze dehydrated tuna muscle are -74 degrees C and 79% (w/w), respectively. 相似文献
18.
29 kDa Trypsin from the pyloric ceca of Atlantic Bonito (Sarda sarda): recovery and characterization
Klomklao S Benjakul S Visessanguan W Kishimura H Simpson BK 《Journal of agricultural and food chemistry》2007,55(11):4548-4553
Trypsin from the pyloric ceca of Atlantic bonito (Sarda sarda) was purified and characterized with respect to its purity; molecular weight; sensitivity to temperature, pH, and inhibition; and N-terminal sequence. The purified trypsin had a molecular weight of 29 kDa as per sodium dodecyl sulfate polyacrylamide gel electrophoresis, and optimal activity was observed at pH 9 and 65 degrees C with BAPNA as a substrate. The enzyme was stable to heat treatment up to 50 degrees C and within the pH range of 7-12. It was stabilized by calcium ions, but its activity was strongly inhibited by soybean trypsin inhibitor, N-p-tosyl-L-lysine chloromethyl ketone, and phenyl methyl sulfonyl fluoride. The enzyme exhibited a progressive decrease in activity with increasing NaCl concentration (0-30%). The N-terminal 20 amino acid residues of Atlantic bonito trypsin were determined as IVGGYECQAHSQPWQPVLNS and were homologous with other trypsins. 相似文献
19.
Yin S Faustman C Tatiyaborworntham N Ramanathan R Maheswarappa NB Mancini RA Joseph P Suman SP Sun Q 《Journal of agricultural and food chemistry》2011,59(22):12198-12203
The effect of the lipid oxidation product, 4-hydroxy-2-nonenal (HNE), on oxidation of oxymyoglobin (OxyMb) from seven different meat-producing species was investigated. Relative to controls, HNE increased OxyMb oxidation within all species (p < 0.05) at both 25 and 4 °C, pH 5.6. The relative effect of HNE was greater for myoglobins (Mbs) that contained 12 ± 1 histidine (His) residues than for those that contained 9 His residues (p < 0.05); HNE efficacy in all species except chicken and turkey decreased with time. Mono-HNE adducts were detected in all species except chicken and turkey. In general, HNE alkylation increased the Mbs' ability to accelerate lipid oxidation in a microsome model. However, neither an HNE nor a Mb species dependent effect was observed. Results suggested that microsome model system associated lipid oxidation overshadowed HNE and species effects on OxyMb oxidation observed in lipid-free systems. 相似文献
20.
Huang TC Huang YW Hung HJ Ho CT Wu ML 《Journal of agricultural and food chemistry》2007,55(13):5097-5102
Proline dehydrogenase (PRODH) catalyzes the biosynthesis of Delta1-pyrroline-5-carboxylic acid (P5C). The Bacillus subtilis subsp. natto gene for the proline dehydrogenase (BnPRODH) was cloned and expressed in Escherichia coli. Nucleotide sequence analysis of the clone revealed an open-reading frame that encodes 302 amino acid polypeptide with a calculated molecular mass of 34.5 kDa. The deduced amino acid sequence showed sequence similarity to bacterial PRODH and PutA of E. coli. The BnPRODH gene was cloned into pET21b and was expressed at a high level in E. coli BL21(DE3). The expressed protein was purified by using nickel ion affinity column chromatography to homogeneity before characterization. The purified recombinant BnPRODH was used to produce P5C. Model system composed of P5C and methylglyoxal was set up to study the formation of 2-acetyl-1-pyrroline. Our data showed that P5C, derived from the conversion of l-proline by the purified recombinant PRODH, might react directly with methylglyoxal to form 2-AP. P5C/methylglyoxal pathway represents the first report of a biological mechanism by which 2-AP may be synthesized in vitro by PRODH. 相似文献