Your search keyword '"purification"' showing total 233 results

1. The improved purification technique for isolation of the novel CGTase from the alkaliphilc strain <italic>Caldalkalibacillus mannanilyticus</italic> IB-OR17-B1.

Author

Yu. Milman, P., Gilvanova, E. A., and Aktuganov, G. E.

Subjects

*SORPTION techniques, *ION exchange chromatography, *CHEMICAL industry, *BIOTECHNOLOGY industries, *ULTRAFILTRATION

Abstract

AbstractCyclodextrin-glucanotransferase (CGTase, EC 2.4.1.19) is a multifunctional enzyme that catalyzes many enzymatic reactions including cyclization, binding, disproportionation and hydrolysis reactions, playing an important role in the enzymatic synthesis of compounds that are widely used in agriculture, pharmaceuticals, food, chemical and biotechnology industries. The present research is aimed to optimize the purification protocol for the extracellular CGTase of alkaliphilc bacterial strain Caldalkalibacillus mannanilyticus IB-OR17-B1 guaranteeing the enzyme homogeneity and its high yield. The improved combination of ultrafiltration and corn-starch (5% w/v) affinity sorption techniques resulted to mild and rapid isolation of electrophoritically homogenic enzyme at 18 × increase of its specific activity and yield 56%. The developed two-step procedure instead the practiced tree-step one using commonly ion-exchange chromatography as final purification technique highly contributes in advance of cost-effectiveness for industrial production and isolation of valuable CGTases. [ABSTRACT FROM AUTHOR]

Published

2024

2. Optimization of total flavonoids purification process in rose by uniform design method.

Author

Qin, Dongmei, He, Cui, Gao, Yuefeng, and Lyu, Bo

Subjects

*FLAVONOIDS, *RATE setting, *ADSORPTION capacity, *ROSES, *DESORPTION

Abstract

This study aims to establish a method for purifying total flavonoids in roses using macroporous resin columns, intending to leverage and harness their potential. We screened six macroporous resins to evaluate their capacity for their adsorption and desorption, ultimately identifying X5 macroporous resin as the most effective. To comprehensively understand the adsorption behavior, we analyzed it using various models, such as pseudo-first-order and pseudo-second-order kinetic models, particle diffusion models, and Langmuir, Freundlich, and Temkin isotherm models. Employing both single-factor and uniform design, approaches, the focus of this work was on maximizing the total flavonoid recovery rate. A 3-factor and 10-level uniform design table was utilized for optimizing the optimal process parameters and exploring the antioxidant properties of the purified flavonoids. The optimal process conditions for purifying total flavonoids from roses can be summarized as follows: a sample concentration of 2 mg/mL, pH at 2, 55 mL sample volume, eluent ethanol concentration of 75%, eluent volume of 5 BV, and the elution rate set at 1 mL/min. Following purification, the total flavonoid content peaked at 57.82%, achieving an 84.93% recovery rate, signifying substantial antioxidant potential. Consequently, the method established for purifying TFR using X5 macroporous resin in this study proves to be a dependable and reliable method consistent approach. [ABSTRACT FROM AUTHOR]

Published

2024

3. Purification and biochemical characterization of novel α-amylase and cellulase from Bacillus sp. PM06.

Author

Rajesh, Rekha and Gummadi, Sathyanarayana N.

Subjects

*CELLULASE, *AMYLASES, *BACILLUS (Bacteria), *WHEAT bran, *CARBOXYMETHYLCELLULOSE, *AMYLOLYSIS, *AMMONIUM sulfate, *BIOCHEMICAL substrates

Abstract

Bacillus sp. PM06, previously isolated from sugarcane waste pressmud, could produce dual enzymes α-amylase and cellulase. The isolate's crude enzymes were purified homogeneously using ammonium sulfate precipitation followed by High Quaternary amine anion exchange chromatography. Purified enzymes revealed the molecular weights of α-amylase and cellulase as 55 and 52 kDa, with a purification fold of 15.4 and 11.5, respectively. The specific activity of purified α-amylase and cellulase were 740.7 and 555.6 U/mg, respectively. It demonstrated a wide range of activity from pH 5.0 to 8.5, with an optimum pH of 5.5 and 6.4 for α-amylase and cellulase. The optimum temperature was 50 °C for α-amylase and 60 °C for cellulase. The kinetic parameters of purified α-amylase were 741.5 ± 3.75 µmol/min/mg, 1.154 ± 0.1 mM, and 589 ± 3.5/(smM), using starch as a substrate. Whereas cellulase showed 556.3 ± 1.3 µmol/min/mg, 1.78 ± 0.1 mM, and 270.9 ± 3.8/(smM) of Vmax,Km, Kcat/Km, respectively, using carboxymethyl cellulose (CMC) as substrate. Among the various substrates tested, α-amylase had a higher specificity for amylose and CMC for cellulase. Different inhibitors and activators were also examined. Ca2+ Mg2+, Co2+, and Mn2+ boosted α-amylase and cellulase activities. Cu2+ and Ni2+ both inhibited the enzyme activities. Enzymatic saccharification of wheat bran yielded 253.61 ± 1.7 and 147.5 ± 1.0 mg/g of reducing sugar within 12 and 24 h of incubation when treated with purified α-amylase and cellulase. A more significant amount of 397.7 ± 1.9 mg/g reducing sugars was released from wheat bran due to the synergetic effect of two enzymes. According to scanning electron micrograph analysis, wheat bran was effectively broken down by both enzymes. [ABSTRACT FROM AUTHOR]

Published

2024

4. Expression and characterization of an organic solvent tolerant recombinant lipase from Staphylococcus capitis SH6 for food wastewater treatment.

Author

Rmili, Fatma, Krayem, Najeh, Loiseau, Celine, Gauvry, Laurent, Frikha, Fakher, Ergan, Françoise, Chamkha, Mohamed, Sayari, Adel, and Fendri, Ahmed

Subjects

*LIPASES, *ORGANIC solvents, *WASTEWATER treatment, *AMINO acid sequence, *AMINO acid residues, *FAST food restaurants

Abstract

The study illustrated here aims on an organic solvent tolerant lipase from Staphylococcus capitis (SCL). The gene part, encoding the mature lipase, was cloned and sequenced. The concluded polypeptide sequence, equivalent to the protein, consist of 388 amino acid residues with a molecular mass of about 45 kDa. A structure-based alignment of the SCL amino acid sequence shows high identities with those many staphylococcal lipases. From this alignment of sequences, the catalytic triad (Ser 117, Asp 308 and His 347) of SCL could be identified. The mature part of the SCL was expressed in Escherichia coli and the recombinant lipase (r-SCL) was purified to homogeneity. The purified r-SCL presented a quite interesting stability at low temperatures (< 30 °C) and the enzyme was found to be highly stable in polar organic solvent and at a pH ranging from 3 to 12. After that, we have demonstrated that the recombinant enzyme may be implicated in the biodegradability of oily wastewater from effluents of fast-food restaurants; the maximum conversion yield into fatty acids obtained at 30 °C, was 65%. [ABSTRACT FROM AUTHOR]

Published

2024

5. Optimization and purification of laccase activity from Mammaliicoccus sciuri isolated from the soils of Similipal, Odisha, India: a kinetics study of crystal violet dye decolorization.

Author

Mahuri, Monalisa, Mohanty, Monalisa, and Thatoi, Hrudayanath

Subjects

*GENTIAN violet, *LACCASE, *METHYLENE blue, *AMMONIUM sulfate, *BIOSPHERE reserves, *SOILS

Abstract

Four laccase-producing bacteria were found in soil samples from the Similipal Biosphere Reserve in Odisha, according to the current study. The isolates (SLCB1 to SLCB4) were evaluated for their laccase-producing ability in LB broth supplemented with guaiacol. The ABTS assay was performed to assess the laccase activity. The bacterium Mammaliicoccus sciuri shows the highest laccase activity i.e., 0.5125 U/L at the optimized conditions of pH 5.5, temperature 32.5 °C, ABTS concentration of 0.75 μl with an incubation time of 9 d. Laccase activity of M. sciuri grown in Sawdust was significantly increased in comparison to that in other agro wastes. The partially purified laccase enzyme after ammonium sulfate precipitation and dialysis showed a molecular weight of ∼58.5 kDa as determined by SDS-PAGE. A decolorization efficiency of 66.67% was recorded for the dye crystal violet after 1 h treatment with dialyzed laccase enzyme compared with phenol red, brilliant blue, and methylene blue. [ABSTRACT FROM AUTHOR]

Published

2024

6. Enhancement in T1 lipase purification recovery using the novel construct pGEX4T1/His-T1.

Author

Hussian, Che Haznie Ayu Che, Rahman, Raja Noor Zaliha Raja Abd, Leow, Adam Thean Chor, Salleh, Abu Bakar, Ali, Mohd Shukuri Mohamad, and Latip, Wahhida

Subjects

*LIPASES, *SITE-specific mutagenesis, *ION exchange (Chemistry), *ESCHERICHIA coli, *SEPHAROSE

Abstract

The Geobacillus zalihae strain T1 produces a thermostable T1 lipase that could be used for industrial purposes. Previously, the GST-T1 lipase was purified through two chromatographic steps: affinity and ion exchange (IEX) but the recovery yield was only 33%. To improve the recovery yield to over 80%, the GST tag from the pGEX system was replaced with a poly-histidine at the N-terminal of the T1 lipase sequence. The novel construct of pGEX/His-T1 lipase was developed by site-directed mutagenesis, where the XbaI restriction site was introduced upstream of the GST tag, allowing the removal of tag via double digestion using XbaI and EcoRI (existing cutting site in the pGEX system). Fragment of 6 × His-T1 lipase fusion was synthesized, cloned into the pGEX4T1 system, and expressed in Escherichia coli BL21 (DE3) pLysS, resulting in lipase-specific activity at 236 U/mg. The single purification step of His-T1 lipase was successfully achieved using nickel Sepharose 6FF with an optimized concentration of 5 mM imidazole for binding, yielding the recovery of 98%, 1,353 U/mg lipase activity, and a 5.7-fold increase in purification fold. His-T1 lipase was characterized and was found to be stable at pH 5–9, active at 70 °C, and optimal at pH 9. [ABSTRACT FROM AUTHOR]

Published

2024

7. High-level production and purification of bioactive recombinant human activin A in Chinese hamster ovary cells.

Author

Kim, Changin, Kim, Hyunjoo, Park, Jeong Soo, Park, Jiwon, Oh, Jeongmin, Yoon, Jaeseung, and Baek, Kwanghee

Subjects

*CHO cell, *ACTIVIN, *BIODIVERSITY

Abstract

Activin A, a member of the TGF-β superfamily, is a homodimer of the inhibin βΑ subunit that plays a diversity of roles in biological processes. Because of its multiple functions, significant efforts have been made to produce activin A, however, unsatisfactory results were obtained due to its low level of expression. In this study, a stable CHO cell line exhibiting high expression of rhActivin A was isolated and production of rhActivin A was achieved using the cell line from 11-day fed-batch cultures in a 7.5 L bioreactor. The production rate was 0.22 g/L, substantially higher than those reported in previous studies. The culture supernatant of the bioreactor was used to purify rhActivin A (purity: >99%, recovery rate: 47%). The purified rhActivin A exhibited biological activity, with an EC50 of 3.893 ng/mL and a specific activity of 1.38 × 103 IU/mg. The control of process-related impurities in the purified rhActivin A was successful and met the USP recommendations for use in cell therapy. Thus, our production and purification methods were appropriate for large-scale GMP-grade rhActivin A production, which can be used for various purposes including cell therapy. [ABSTRACT FROM AUTHOR]

Published

2024

8. Factors affecting therapeutic protein purity and yield during chromatographic purification.

Author

Che Hussian, Che Haznie Ayu and Leong, Wai Yie

Subjects

*RECOMBINANT proteins, *PROTEIN fractionation, *RECOMBINANT DNA, *PROTEINS, *ANIMAL health

Abstract

Therapeutic proteins are recombinant proteins generated through recombinant DNA technology and have attracted a great deal of interest in numerous applications, including pharmaceutical, cosmetic, human and animal health, agriculture, food, and bioremediation. Producing therapeutic proteins on a large scale, mainly in the pharmaceutical industry, necessitates a cost-effective, straightforward, and adequate manufacturing process. In industry, a protein separation technique based mainly on protein characteristics and modes of chromatography will be applied to optimize the purification process. Typically, the downstream process of biopharmaceutical operations may involve multiple chromatography phases that require the use of large columns pre-packed with resins that must be inspected before use. Approximately 20% of the proteins are assumed to be lost at each purification stage during the production of biotherapeutic products. Hence, to produce a high quality product, particularly in the pharmaceutical industry, the correct approach and understanding of the factors influencing purity and yield during purification are necessary. [ABSTRACT FROM AUTHOR]

Published

2024

9. Purification of lipase from Burkholderia metallica fermentation broth in a column chromatography using polymer impregnated resins.

Author

Ng, Zhang Jin, Abbasiliasi, Sahar, Yew Joon, Tam, Ng, Hui Suan, Phapugrangkul, Pongsathon, and Tan, Joo Shun

Subjects

*LIPASES, *COLUMN chromatography, *POLYMERS, *BURKHOLDERIA, *GLASS beads, *SODIUM acetate

Abstract

In this work, porous glass beads grafted with polyethylene glycol (PEG) were used as an adsorbent to purify lipase from Burkholderia metallica in column chromatography. The purification parameters viz. salt stability, types and concentrations of PEG and salt, pH of the binding solution, and flow rate were studied to determine the performance of the purification system in an XK16/20 column. The crude lipase was mixed with different types and concentrations of salts 1–5% (w/w) (sodium citrate, potassium citrate, and sodium acetate) and subjected to the column containing the polymeric glass bead. One-variable-at-a-time experimentation revealed that 20% (w/w) PEG 6000 g/mol impregnated glass beads with a binding solution of 5% sodium citrate at pH 7.7, a flow rate of 1.0 mL/min and extraction time of 10 min resulted in the highest purification factor and recovery yield at 3.67 and 88%, respectively. The purified lipase has 55 ∼ 60 kDa molecular mass. The outcome of the study showed PEG could be applied to modify the inert glass beads into polymeric form, providing a biocompatible and mild separation condition for lipase. Thus, PEG could be successfully applied for the purification of lipase from B. metallica fermentation broth using column chromatography. [ABSTRACT FROM AUTHOR]

Published

2023

10. Cost-effective, high-yield production of Pyrobaculum calidifontis DNA polymerase for PCR application.

Author

Maseh, Kashif, Ali, Syed Farhat, Ahmad, Shazeel, and Rashid, Naeem

Subjects

*DNA polymerases, *AFFINITY chromatography, *POLYMERASE chain reaction, *GENETIC engineering, *MOLECULAR cloning, *GENE expression, *THAWING

Abstract

Polymerase Chain Reaction (PCR) is widely used for cloning, genetic engineering, mutagenesis, detection and diagnosis. A thermostable DNA polymerase is required for PCR. Here we describe low-cost and high-recovery production of Pyrobaculum calidifontis DNA polymerase (Pca-Pol). The gene was cloned in pET-28a and expressed in Escherichia coli BL21CodonPlus. Gene expression conditions were optimized. Eventually, gene expression was induced with 0.1 mM IPTG for 3 hours at 37 °C. Recombinant Pca-Pol produced was purified to homogeneity by immobilized metal-ion affinity chromatography yielding around 9000 U of Pca-Pol per liter of the culture with a recovery of 92%. Stability and PCR amplification efficiency of Pca-Pol was tested under various storage conditions with highest efficiency in 25 mM Tris-Cl buffer (pH 8.5) containing 0.1% Tween 20, 0.2 mg/mL BSA and 20% glycerol. Under this condition, no loss in PCR activity of Pca-Pol was observed, even after one year of storage. Repeated freeze-thaw, however, deteriorated enzyme activity of Pca-Pol. 55% PCR amplification activity retained after 7 prolong freeze-thaw cycles (freezing overnight at −20 °C and thawing for 45 minutes at 28 °C). Purified Pca-Pol possessed 3′–5′ exonuclease (proofreading) activity and is expected to have greater fidelity as compared to Taq polymerase which does not have proofreading activity. [ABSTRACT FROM AUTHOR]

Published

2023

11. Bioprocessing and purification of extracellular L-asparaginase produced by endophytic Colletotrichum gloeosporioides and its anticancer activity.

Author

Yap, Ling Sze, Lee, Wai Leng, and Ting, Adeline Su Yien

Subjects

*ANTINEOPLASTIC agents, *COLLETOTRICHUM gloeosporioides, *GEL permeation chromatography, *RESPONSE surfaces (Statistics), *LYMPHOBLASTIC leukemia, *WESTERN immunoblotting

Abstract

L-asparaginase is an enzyme commonly used to treat acute lymphoblastic leukemia. Commercialized bacterial L-asparaginase has been reported to cause several life-threatening complications during treatment, hence the need to seek alternative sources of L-asparaginase. In this study, the novelty of upstream and downstream bioprocessing of L-asparaginase from a fungal endophyte, Colletotrichum gloeosporioides, and the cytotoxicity evaluation was demonstrated. Six variables (carbon source and concentration, nitrogen source and concentration, incubation period, temperature, pH and agitation rate) known to influence L-asparaginase production were studied using One-Factor-At-A-Time (OFAT) approach, with four significant variables further optimized using Response Surface Methodology (RSM). The crude extract produced using optimized condition was purified, characterized and examined for its anticancer effect. Purification of fungal L-asparaginase was performed via ultrafiltration and size exclusion chromatography, which are less common techniques. The protein profile and monomeric weight of L-asparaginase were determined using SDS-PAGE and Western blot. Cytotoxicity of purified L-asparaginase on leukemic Jurkat E6 and oral carcinoma cells were studied using MTS assay for 24 h and 48 h. OFAT results from optimization showed that glucose and L-asparagine concentrations, incubation period and temperature, were significant factors affecting L-asparaginase production by C. gloeosporioides. RSM analysis further evidence the significant interaction between glucose and L-asparagine concentrations in inducing L-asparaginase production. Purified L-asparaginase was profiled with specific activity of 255.02 IU/mg protein, purification fold of 6.12, and 34.63% of enzyme recovery. SDS and Western blot revealed that the purified L-asparaginase might be a tetramer with monomeric units of 25 kDa. Purified L-asparaginase was discovered to be more efficient against Jurkat leukemic cells than against H103 oral carcinoma cells, as lower IC50 value was observed for Jurkat cell lines (46.36 ± 1.52 µg/mL for Jurkat and 125.56 ± 7.28 µg/mL for H103). In short, purified L-asparaginase derived from endophytic C. gloeosporioides showed high purity and significant anticancer effect toward cancer cells. This study therefore demonstrated the potential of fungal L-asparaginase as alternative chemotherapy drug in the future. [ABSTRACT FROM AUTHOR]

Published

2023

12. Purification and biochemical characterization of catalase that confers protection against hydrogen peroxide induced by stressful desert environment: the Camelus Dromedarius kidney catalase.

Author

Chafik, Abdelbasset, Essamadi, Abdelkhalid, Çelik, Safinur Yildirim, and Mavi, Ahmet

Subjects

*CATALASE, *CAMELS, *LIGAND exchange chromatography, *HYDROGEN peroxide, *POISONS, *PSYCHOLOGICAL stress

Abstract

Camel is continually exposed to stressful desert environment that enhances generation of reactive oxygen species, including hydrogen peroxide (H2O2). Catalase plays an important role in detoxification of H2O2. A highly active catalase from camel kidney was purified to homogeneity, with a specific activity of 1,774,392 U/mg protein, using ion exchange and metal chelate affinity chromatography. The molecular weight of the enzyme was 268 kDa consisting of four identical subunits of 63 kDa. The enzyme showed higher optimum temperature (45 °C) and higher activation energy (4.37 kJ mol−1). The thermodynamic parameters, ΔH, ΔG and ΔS, were determined. The effect of various metal ions and chemicals on enzyme activity was investigated. Km, Vmax, kcat and kcat/Km values for H2O2 were found to be 46 mM, 10,715,045 U/mg, 48,265,968 s−1 and 2,966,562 s−1 mM−1, respectively. Camel kidney catalase displayed higher affinity efficiency for H2O2 and can protect reduced glutathione (GSH) from oxidation by H2O2. Sodium azide was found to be a noncompetitive inhibitor of enzyme with Ki and IC50 of 17.88 µM and 20.94 µM, respectively. Camel catalase showed unique biochemical properties. Interestingly, camel catalase can protect molecules (GSH) and organ functions (kidney) from the toxic effects of H2O2 induced by stressful desert environment. [ABSTRACT FROM AUTHOR]

Published

2023

13. Three-phase partitioning, a recyclable method for the purification of R-phycoerythrin from a red algae Porphyra yezoensis.

Author

Wang, Quanfu, Zhang, Qingyu, Zhang, Ailin, and Hou, Yanhua

Subjects

*RED algae, *PORPHYRA, *BANGIALES, *FLUORESCENCE spectroscopy, *TEMPERATURE effect

Abstract

In this study, R-phycoerythrin (R-PE) was isolated and characterized from Porphyra yezoensis by three-phase partitioning (TPP) method. The effects of temperature, time, pH, salt saturation, and volume ratio on the purity and recovery rate of R-PE were studied. The optimum extraction conditions were determined as follows: salt saturation of 70%, temperature of 25 °C, time of 45 min, pH of 7.0, and volume ratio of 1:1. Under the optimal extraction conditions, the purity of R-PE was 3.90. The results of SDS-PAGE showed that R-PE has three bands at 23 kDa, 22 kDa, and 18 kDa, corresponding to its α, β, γ subunits. The structure and optical activity of R-PE did not change before and after purification based on ultraviolet, infrared, and fluorescence spectra. In addition, the purity and recovery rate of R-PE extracted by tert-butanol were evaluated. The results showed that the extraction performance of tert-butanol for R-PE remained unchanged in three recoveries. These show that TPP is an efficient, green, and recyclable extraction technology. [ABSTRACT FROM AUTHOR]

Published

2023

14. Purification and characterization of chitinase produced by thermophilic fungi Thermomyces lanuginosus.

Author

Suryawanshi, Nisha and Eswari, J. Satya

Subjects

*CHITIN, *CHITINASE, *THERMOPHILIC fungi, *GEL permeation chromatography, *ION exchange chromatography, *AMMONIUM sulfate

Abstract

In the past few years, the production of shrimp shell waste from the seafood processing industries has confronted a significant surge. Furthermore, insignificant dumping of waste has dangerous effects on both nature and human well-being. This marine waste contains a huge quantity of chitin which has several applications in different fields. The chitinase enzyme can achieve degradation of chitin, and the chitin itself can be used as the substrate as well for production of chitinase. In the current study, the chitinase enzyme was produced by Thermomyces lanuginosus. The extracellular chitinase was purified from crude extract using ammonium sulfate precipitation followed by DEAE-cellulose ion-exchange chromatography and Sephadex G-100 gel filtration chromatography. The stability and activity of chitinase with different pH, temperature, different times for a reaction, in the presence of different metal ions, and different concentration of enzyme and substrate were analyzed. The chitinase activity was found to be highest at pH 6.5, 50 °C, and 60 min after the reaction began. and the chitinase showed the highest activity and stability in the presence of β-mercaptoethanol (ME). The SDS-PAGE of denatured purified chitinase showed a protein band of 18 kDa. The characterization study concludes that Cu2+, Hg2+, and EDTA have an inhibitory effect on chitinase activity, whereas β-ME acts as an activator for chitinase activity. The utilization of chitin to produce chitinase and the degradation of chitin using that chitinase enzyme would be an opportunity for bioremediation of shrimp shell waste. [ABSTRACT FROM AUTHOR]

Published

2022

15. Production, purification and characterization of a novel antithrombotic and anticoagulant serine protease from food grade microorganism Neurospora crassa.

Author

Duan, Yajie, Katrolia, Priti, Zhong, Ailing, and Kopparapu, Narasimha Kumar

Subjects

*NEUROSPORA crassa, *FIBRINOLYTIC agents, *PLASMINOGEN activators, *HEPARIN, *TRYPSIN inhibitors, *MOLECULAR weights, *SERINE proteinases, *PROTEOLYTIC enzymes

Abstract

A novel thrombolytic enzyme was produced by food grade microorganism Neurospora crassa using agro-industrial by-products as substrates. Process parameters were optimized using Plackett–Berman and Box–Benhken design. Under the optimized fermentation conditions, high fibrinolytic activity of 403.59 U/mL was obtained. It was purified with a specific activity of 3572.4 U/mg by ammonium sulfate precipitation and SP Sepharose chromatography. The molecular weight of the enzyme was approximately 32 kDa. It exhibited maximum activity at 40 °C and pH 7.4. Its activity was enhanced by Cu2+, Na+, Zn2+, and completely inhibited by phenylmethanesulfonyl fluoride, soybean trypsin inhibitor, aprotinin, which indicates it could be a serine protease. The enzyme could degrade fibrin clot directly without the need of plasminogen activator, and effectively cleaved Aα, Bβ, γ chains of fibrinogen. It could inhibit the formation of blood clots in vitro and acts as an anticoagulant. Compared to heparin the purified enzyme showed extended anticoagulant activity. Blood clots were dissolved effectively and dissolution rate was increased with time. Based on these results, this novel enzyme has the potential to be developed as a thrombolytic agent. [ABSTRACT FROM AUTHOR]

Published

2022

16. Biochemical studies of enzyme-induced browning of African bush mango (Irvingia gabonensis) fruit pulp.

Author

Adeseko, Catherine Joke, Sanni, David Morakinyo, and Lawal, Olusola Tosin

Subjects

*MANGO, *FRUIT, *TEMPERATURE control, *ENZYME inactivation, *MOLECULAR weights, *POLYPHENOL oxidase

Abstract

The purpose of this study was to examine the biochemical properties of African bush mango (Irvingia gabonensis) pulp PPO. PPO was purified from I. gabonensis fruit pulp in three steps and characterized. A purification fold of 343 with specific activity of 216 U/mg and 13% recovery were obtained as well as molecular weight of 32.67 kDa was observed. The optimum pH and temperature were found to be pH 7.0 and 50 °C respectively while the enzyme showed instability at low pH 2–4 with total inactivation at pH 2 but maximal at pH 5–9 with remaining residual activity of 60–90%, whereas, total enzyme activity inactivation was observed at 90 °C. However, Cu2+, Fe2+ and Mg2+ enhanced the PPO activity but inhibited by Ca2+, Ba2+, K+ and Na+. Notably, purified PPO was inactivated completely by urea at concentration above 10 mM while Km and Vmax values were estimated to be 7.34 mM and 0.36 U/min for catechol, 10.76 mM and 0.30 U/min for L-DOPA, and 14.90 mM and 0.26 U/min for tyrosine, respectively. The activity of PPO in I. gabonensis fruit and its juicy product could be controlled at high temperature in acidified medium. [ABSTRACT FROM AUTHOR]

Published

2022

17. Extraction and purification of Aspergillus tamarii β-fructofuranosidase with transfructosylating activity using aqueous biphasic systems (PEG/phosphate) and magnetic field.

Author

de Oliveira, Rodrigo Lira, Bernardino, Maria Itais dos Santos, Silva, Talis Bruno Santos, Converti, Attilio, Porto, Camila Souza, and Porto, Tatiana Souza

Subjects

*MAGNETIC fields, *POLYETHYLENE glycol, *MAGNETIC flux density, *ASPERGILLUS, *MAGNETICS, *PARTITION coefficient (Chemistry), *INSULIN aspart, *FRUCTOOLIGOSACCHARIDES

Abstract

β-fructofuranosidases (FFases) are enzymes involved in sucrose hydrolysis and fructo-oligosaccharides' production which are of great interest for the food industry. FFase from Aspergillus tamarii URM4634 was extracted using PEG/Phosphate Aqueous Biphasic Systems (ABS), and the impact of magnetic field on the extraction behavior was evaluated. A 24-full experimental design was employed to study the influence of molar mass of PEG, concentrations of PEG and phosphate and pH on the selected response variables, i.e., partition coefficient (K), purification factor (PF), activity yield (Y) and selectivity (S). The influence of magnetic field during partition and NaCl concentration on the same responses was also studied. The best results of FFase extraction without magnetic field (K = 0.50, PF = 4.05, Y = 72.66% and S = 0.06) were observed at pH 8.0 using 12.5% (w/w) PEG 400 and 25% (w/w) NaH2PO4/K2HPO4. Application of the magnetic field allowed improving the performance, with the best results being obtained at the longest distance between magnets (lowest magnetic field) and absence of NaCl (K = 0.93, PF = 4.22, Y = 83.79% and S = 0.09). The outcomes obtained demonstrate that ABS combination with low intensity magnetic field can be used as an efficient FFase pre-purification method. [ABSTRACT FROM AUTHOR]

Published

2022

18. Optimization of fermentation conditions, purification and rheological properties of poly (γ-glutamic acid) produced by Bacillus subtilis 1006-3.

Author

Zhang, Ruoshi, Zhang, Shihao, Jiang, Guangyang, Gan, Longzhan, Xu, Zhe, and Tian, Yongqiang

Subjects

*RHEOLOGY, *BACILLUS subtilis, *NON-Newtonian fluids, *PSEUDOPLASTIC fluids, *AMINO acid analysis

Abstract

This study aimed to investigate the optimal fermentation condition, purification and rheological properties of extracellular polymers produced by Bacillus subtilis 1006-3. An optimum temperature of 30.2 °C, inoculation amount of 6.1%, and pH of 8.2 were determined via Response Surface Methodology. The result of amino acid analysis and gel electrophoresis indicated that the obtained polymer contained only glutamic acid, with a wide molecular weight range. This polymer was finally determined as γ-PGA by infrared spectroscopy. The γ-PGA solution displayed a behavior of pseudoplastic non-Newtonian fluid with shear thinning properties, which can be described by the Ostward-de Waele power law model. The apparent viscosity of γ-PGA solution increased with the increase in its concentration from 1% to 10%. The deviation in pH from neutral value, and the addition of NaCl or MgCl2 can reduce the apparent viscosity of γ-PGA solution, and it was more sensitive to Mg2+ than to Na+ addition. At the concentration of 4, 6, and 8%, γ-PGA solution showed predominantly viscous response in the range of 0.1–100 rad/s angular frequency (G″>G′). These results indicated the potential application of the γ-PGA as a thickening agent. [ABSTRACT FROM AUTHOR]

Published

2022

19. Optimization for the extraction of polyphenols from Inonotus obliquus and its antioxidation activity.

Author

Wang, Yu, Ouyang, Fengju, Teng, Chunying, and Qu, Juanjuan

Subjects

*PROCYANIDINS, *PLANT polyphenols, *GALLIC acid, *POLYPHENOLS, *HIGH performance liquid chromatography, *CAFFEIC acid, *HYDROXYL group, *OXIDANT status

Abstract

In order to study the extraction process and antioxidative activity of Inonotus obliquus polyphenols (IOP), the optimal extraction process was determined by orthogonal experiment optimization. The clearance rate of DPPH and hydroxyl radicals were used as indicators to evaluate the antioxidant activity of IOP. The results showed that the optimum extraction conditions were as follows: ethanol concentration of 50%, solid–liquid ratio of 1:20, temperature of 60 °C, and 90 min. Under these conditions, the extraction yield of IOP was 2.84%. The antioxidant capacity of extracts appeared to be IOP dose-dependent, while it also presented stronger ferric reducing antioxidant power (FRAP). High Performance Liquid Chromatography (HPLC-MS) analysis indicated that the major identified polyphenol compounds extracted at the optimal conditions were ten compounds (procyanidin, caffeic acid, p-coumaric acid, isorhamnetin-3-O-glucoside, astilbin, tangeretin, gallic acid, kaempferol, quercetin, and catechin 7-xyloside). These findings indicate that I. obliquus polyphenols have the potential to be developed as a natural antioxidant and have a good application prospect. [ABSTRACT FROM AUTHOR]

Published

2021

20. Biochemical characterization of a partially purified protease from Aspergillus terreus 7461 and its application as an environmentally friendly dehairing agent for leather industry.

Author

de Lima, Emmly Ernesto, Franco, Daniel Guerra, Galeano, Rodrigo Mattos Silva, Guimarães, Nelciele Cavalieri de Alencar, Masui, Douglas Chodi, Giannesi, Giovana Cristina, and Zanoelo, Fabiana Fonseca

Subjects

*LEATHER industry, *ASPERGILLUS terreus, *WHEAT bran, *HAIR removal, *REDUCING agents, *PROTEOLYTIC enzymes

Abstract

Proteases can be used in several biotechnological processes including detergent, food and leather industries. In the leather industry, dehairing is carried out by chemicals, which pollute the environment. Therefore, to make the hair removal process environmentally friendly, a protease produced by Aspergillus terreus has been purified, biochemically characterized and had an efficient ability to remove hair from bovine leather. The protease was produced using 1% wheat bran and was purified 2.3-fold using two chromatographic steps showing a molecular weight of 90 kDa. Optimal temperature and pH were 50 °C and 6.5, respectively. Thermal stability was up to 1 h at 50 °C. Protease was stable to detergents like Tween 80 and to organic solvents. The activity was activated by Ca2+ and inhibited by Hg2+ and Cu2+. The enzyme was classified as serine protease, by the inhibition by PMSF and was stable to reducing agents. It hydrolyzed casein, azocasein, BSA, egg albumin and BTpNA. The Km and Vmax values were 0.65 ± 0.03 mg/mL and 3.66 ± 0.18 μmol/min, respectively. Remarkable properties about temperature, pH, stability to detergents and reducing agents ensure that the protease from A. terreus can be an excellent candidate for industrial applications, particularly in the leather industry. [ABSTRACT FROM AUTHOR]

Published

2021

21. Bioseparation of phycocyanin from Phormidium tergestinum using an aqueous two-phase system.

Author

Tan, Joo Shun, Abbasiliasi, Sahar, Lalung, Japareng, Tam, Yew Joon, Murugan, Paramasivam, and Lee, Chee Keong

Subjects

*PHYCOCYANIN, *POTASSIUM phosphates, *POLYETHYLENE glycol, *MOLECULAR weights, *GEL electrophoresis, *POLYACRYLAMIDE gel electrophoresis, *SODIUM dodecyl sulfate

Abstract

This study aimed at purification of phycocyanin (PC) from Phormidium tergestinum using an aqueous two-phase system (ATPS) comprised of polyethylene glycol (PEG) and salts. The partitioning efficiency of PC in ATPS and the effect of phase composition, pH, crude loading, and neutral salts on purification factor and yield were investigated. Results showed that PC was selectively partitioned toward bottom phase of the system containing potassium phosphate. Under optimum conditions of 20% (w/w) PEG 4000, 10% (w/w) potassium phosphate, 20% (v/v) crude load at pH 7, with addition of 0.5% (w/w) NaCl, PC from P. tergestinum was partially purified up to 5.34-fold with a yield of 87.8%. Sodium dodecyl sulfate-polyacrylamide gel electrophoresis showed that the molecular weight of PC was ∼19 kDa. Results from this study demonstrated ATPS could be used as a potential approach for the purification of PC from P. tergestinum. [ABSTRACT FROM AUTHOR]

Published

2021

22. Novel approach using activated cellulose film for efficient immobilization of purified diamine oxidase to enhance enzyme performance and stability.

Author

Verma, Neelam, Sisodiya, Lovely, Gahlaut, Anjum, Hooda, Vinita, and Hooda, Vikas

Subjects

*ENZYME stability, *IMMOBILIZED enzymes, *PEAS, *POLLUTANTS, *FOOD safety, *CELLULOSE synthase, *GLUTARALDEHYDE, *CELLULOSE

Abstract

The presence of various contaminants in foodstuffs has led to serious public health concerns. Diamine oxidase (DAO) has attracted tremendous attention for guarding food safety as well as clinical and environmental industries. In this study, DAO from Pisum sativum (Pea) seedlings was extracted and purified by dialysis and gel filtration. Purified DAO was covalently immobilized onto the surface of nitrocellulose membrane using glutaraldehyde. The obtained bioaffinity support has efficiently shown high yield immobilization of DAO from pea seedlings. The optimal conditions of free and immobilized DAO activity were evaluated against the substrate, Putrescine dihydrochloride. The influence of pH, temperature, storage stability, and reusability of immobilized enzyme with comparison to the free enzyme was studied and the results showed that the stabilities were significantly enhanced compared with free counterpart. Residual activity of the immobilized enzyme was 59% of the initial activity after being recycled 10 times. We approve that this novel low cost immobilized DAO carrier presents a new approach in large scale applications. [ABSTRACT FROM AUTHOR]

Published

2020

23. Production, optimization, purification, characterization, and anti-cancer application of extracellular L-glutaminase produced from the marine bacterial isolate.

Author

Orabi, Hanaa, El-Fakharany, Esmail, Abdelkhalek, Eman, and Sidkey, Nagwa

Subjects

*SOLID-state fermentation, *MOLECULAR weights, *BACILLUS subtilis, *FACTORS of production, *CHEMICAL industry

Abstract

L-glutaminase from bacterial sources has been proven to be effective and economical agents in cancer therapy, food industry and high-value chemicals like threonine. In the present study, a newly isolated bacterial strain was potentially producing extracellular L-glutaminase, it identified as Bacillus subtilis OHEM11 (MK389501) using the 16S rRNA gene. L-glutaminase production optimized and the optimum factors for production under submerged fermentation were at pH 6.5–7.0 and 35 °C after 28 hr using rhamnose and glutamine as carbon and nitrogen sources, respectively, while bagasse was the best inducer for the production under solid-state fermentation. Ethanol precipitation and ion-exchange chromatography using QFF are the purification steps. L-glutaminase was purified to 2-fold with specific activity 89.78 U/mg and its molecular weight about 54.8 kDa with the alkaline property of the enzyme makes it clear having carcinostatic property; maximum enzyme activity at pH 8.2 and 40 °C and retained about 90% activity for 1 hr. The cytotoxicity effect of L-glutaminase indicated a significant safety on Vero cells with high anticancer activity against NFS-60, HepG-2, and MCF-7 cancer cell lines. The outcomes demonstrated that L-glutaminase could be applied in many biotechnological applications such as pharmaceutical and food processing. [ABSTRACT FROM AUTHOR]

Published

2020

24. High yield expression, characterization, and biological activity of IFNα2-Tα1 fusion protein.

Author

Aslam, Muhammad Shahbaz, Gull, Iram, Mahmood, Malik Siddique, Iqbal, Muhammad Mudassir, Abbas, Zaigham, Tipu, Imran, Ahmed, Aftab, and Athar, Muhammad Amin

Subjects

*CHIMERIC proteins, *WESTERN immunoblotting, *GENE fusion

Abstract

The use of interferon α-2 in combination with thymosin α-1 shows higher anti-cancer effect in comparison when both are used individually because of their synergistic effects. In this study we produced an important human interferon α-2-thymosin α-1 (IFNα2-Tα1) fusion protein with probable pharmaceutical properties coupled to its high-level expression, characterization, and study of its biological activity. The IFNα2-Tα1 fusion gene was constructed by over-lap extension PCR and expressed in Escherichia coli expression system. The expression of IFNα2-Tα1 fusion protein was optimized to higher level and its maximum expression was obtained in modified terrific broth medium when lactose was used as inducer. The fusion protein was refolded into its native biologically active form with maximum yield of 83.14% followed by purification with ∼98% purity and 69% final yield. A band of purified IFNα2-Tα1 fusion protein equal to ∼23 kDa was observed on 12 % SDS-PAGE gel. The integrity of IFNα2-Tα1 fusion protein was confirmed by western blot analysis and secondary structure was assessed by CD spectroscopy. When IFNα2-Tα1 fusion protein was subjected to its biological activity analysis it was observed that it exhibits both IFNα2 & Tα1 activities as well as significantly higher anticancer activity as compared to IFNα-2 alone. [ABSTRACT FROM AUTHOR]

Published

2020

25. Purification and characterization of a propanol-tolerant neutral protease from Bacillus sp. ZG20.

Author

Yu, Ping, Wang, Xinxin, Huang, Xingxing, Ren, Qian, and Yan, Tingting

Subjects

*BACILLUS (Bacteria), *PROTEOLYTIC enzymes, *MOLECULAR weights, *PROPANOLS

Abstract

A propanol-tolerant neutral protease was purified and characterized from Bacillus sp. ZG20 in this study. This protease was purified to homogeneity with a specific activity of 26,655 U/mg. The recovery rate and purification fold of the protease were 13.7% and 31.5, respectively. The SDS-PAGE results showed that the molecular weight of the protease was about 29 kDa. The optimal temperature and pH of the protease were 45 °C and 7.0, respectively. The protease exhibited a good thermal- and pH stability, and was tolerant to 50% propanol. Mg2+, Zn2+, K+, Na+ and Tween-80 could improve its activity. The calculated Km and Vmax values of the protease towards α-casein were 12.74 mg/mL and 28.57 µg/(min mL), respectively. This study lays a good foundation for the future use of the neutral protease from Bacillus sp. ZG20. [ABSTRACT FROM AUTHOR]

Published

2019

26. Purification and characterization of a novel β-glucosidase from Aspergillus flavus and its application in saccharification of soybean meal.

Author

Chen, Zhou, Liu, Yangliu, Liu, Lu, Chen, Yaoyao, Li, Siting, and Jia, Yingmin

Subjects

*GLUCOSIDASES, *SOYBEAN meal, *ASPERGILLUS flavus, *FEED industry, *MOLECULAR weights, *OVERPRODUCTION

Abstract

Aspergillus flavus has been regarded as a potential candidate for its production of industrial enzymes, but the details of β-glucosidase from this strain is very limited. In herein, we first reported a novel β-glucosidase (AfBglA) with the molecular mass of 94.2 kDa from A. flavus. AfBglA was optimally active at pH 4.5 and 60 °C and is stable between pH 3.5 and 9.0 and at a temperature of up to 55 °C for 30 min remaining more than 90% of its initial activity. It showed an excellent tolerance to Trypsin, Pepsin, Compound Protease, and Flavourzyme and its activity was not inhibited by specific certain cations. AfBglA displayed broad substrate specificity, it acted on all tested pNP-glycosides and barley glucan, indicating this novel β-glucosidase exhibited a β-1, 3-1, 4-glucanase activity. Moreover, the AfBglA could effectively hydrolyze the soybean meal suspension into glucose and exhibit a strong tolerance to the inhibition of glucose at a concentration of 20.0 g/L during the saccharification. The maximum amount of the glucose obtained by AfBglA corresponded to 67.0 g/kg soybean meal. All of these properties mentioned above indicated that the AfBglA possibly attractive for food and feed industry and saccharification of cellulolytic materials. [ABSTRACT FROM AUTHOR]

Published

2019

27. Partial characterization of Bacillus pumilus catalase partitioned in poly(ethylene glycol)/sodium sulfate aqueous two-phase systems.

Author

Yuzugullu Karakus, Yonca and Isik, Semih

Subjects

*BACILLUS pumilus, *CATALASE, *HYDROGEN peroxide, *SULFATES, *SODIUM sulfate, *ETHYLENE glycol

Abstract

Aqueous two-phase partitioning system (ATPS) was used to extract and purify catalase from Bacillus pumilus. The system parameters for effective purification of catalase were optimized. The best catalase recovery (123%) with a 4.6-fold purification was obtained in the bottom phase of ATPS including the mixture of 15% (w/w) PEG4000, 10% (w/w) Na2SO4 and 3% (w/w) NaCl at pH 5.0. The purified enzyme was characterized regarding its activity and stability. The highest enzyme activity was observed at pH 7.0 and 37 °C on hydrogen peroxide. The enzyme was quite stable at temperatures between 30 and 55 °C and a pH range of 7.0–9.0. The Km and Vmax values were determined from Lineweaver–Burk plot as 11 mM and 1667 µmole ml−1 min−1, respectively. Overall, it can be said that ATPS is a rapid, reasonable, straightforward and cost-effective process for catalase purification in comparison to the chromatographic methods. [ABSTRACT FROM AUTHOR]

Published

2019

28. Recombinant production of active Streptococcus pneumoniae CysE in E. coli facilitated by codon optimized BL21(DE3)-RIL and detergent.

Author

Verma, Deepali, Antil, Monika, and Gupta, Vibha

Subjects

*STREPTOCOCCUS pneumoniae, *TRITON X-100, *MOLECULAR cloning, *PATHOGENIC bacteria, *KLEBSIELLA pneumoniae, *DRUG resistance

Abstract

The emergence of drug resistance in Streptococcus pneumoniae (Spn) is a global health threat and necessitates discovery of novel therapeutics. The serine acetyltransferase (also known as CysE) is an enzyme of cysteine biosynthesis pathway and is reported to be essential for the survival of several pathogenic bacteria. Therefore, it appears to be a very attractive target for structure–function understanding and inhibitor design. This study describes the molecular cloning of cysE from Spn in the pET21c vector and efforts carried out for expression and purification of active recombinant CysE. Significant expression of recombinant Spn cysE could be achieved in codon optimized BL21(DE3)-RIL strain as opposed to conventional BL21(DE3) strain. Analysis of codon adaptation index (CAI) with levels of eukaryotic genes and prokaryotic cysEs expressed in heterologous E. coli host suggests that codon optimized E. coli BL21(DE3)-RIL may be a better host for expressing genes with low CAI. Here, an efficient protocol has been developed for recovery of recombinant Spn CysE in soluble and biologically active form by the usage of nonionic detergent Triton X-100 at a concentration as low as 1%. Altogether, this study reports a simple strategy for producing functionally active Spn CysE in E. coli. [ABSTRACT FROM AUTHOR]

Published

2019

29. Purification and characterization of lysozyme from Chinese Lueyang black-bone Silky fowl egg white.

Author

Chen, Chen, Li, Xinxin, Yue, Lijuan, Jing, Xian, Yang, Yiqi, Xu, Youmei, Wu, Sanqiao, Liang, Yinku, Liu, Xiang, and Zhang, Xiaoying

Subjects

*LYSOZYMES, *EGG whites, *ION exchange chromatography, *AMINO acid sequence, *AMINO acid residues, *MICROCOCCUS luteus

Abstract

Lysozyme, an important antibacterial protein, is an enzyme that cleaves the glycosidic bond between N-acetylmuramic acid and N-acetylglucosamine of peptidoglycan in cell walls. The novel lysozyme was purified and characterized from Chinese Lueyang black-bone silky fowl (CBSF) egg white, and its N-terminal amino acid sequence, enzymatic properties, and antibacterial activity were investigated. The CBSF lysozyme was purified using adsorption chromatography, ammonium sulfate precipitation, ion exchange chromatography, and size-exclusion chromatography. The purification fold and yield were 3.28 and 14.69%, respectively. The purified lysozyme was revealed as a single protein band with SDS–PAGE and had a MALDI-TOF/TOF molecular weight of 14305.57 Da and a final specific activity of 3.49 × 105 U/mg protein using Micrococcus lysodeikticus as a substrate. The optimum temperature and pH of the lysozyme were 50 °C and 6.0, respectively. The 20 N-terminal amino acid residues of the purified lysozyme were determined to be KVFGRCELAAAMKRHGLDNY, showing some homology to the N-terminus of the odontophoridae egg white lysozyme. The purified lysozyme exerted a potent antimicrobial activity toward indicator microorganisms, including Bacillus subtilis ATCC 6633, Staphylococcus aureus ATCC 25923, and Escherichia coli ATCC 25922. However, its inhibition of gram-negative activity was weaker than that of the Gram-positive bacteria. [ABSTRACT FROM AUTHOR]

Published

2019

30. Construction of Escherichia coli BL21/A-53 producing histidine-tagged carboxymethylcellulase and comparison of its characteristics with CMCase without histidine-tag.

Author

Kang, Duk-Un, Lee, Yong-Suk, and Lee, Jin-Woo

Subjects

*ESCHERICHIA coli, *CARBOXYMETHYLCELLULASE, *HISTIDINE, *MOLECULAR weights, *CELLULOSE, *ENZYME activation

Abstract

To enhance recovery yield of carboxymethylcellulase (CMCase), E. coli BL21/A-53 producing the histidine-tagged CMCase was constructed in this study. The recovery yield of the histidine-tagged CMCase using the His-tag affinity chromatography was 39.8%. The predicted molecular weight of the histidine-tagged CMCase was determined as 56,260 Da. Its Km and Vmax were 9.3 g l−1 and 76.3 g l−1·min−1, respectively. The histidine-tagged CMCase hydrolyzed avicel, carboxymethylcellulose (CMC), filter paper, pullulan, xylan, but there was no detectable activity on cellobiose, p-Nitrophenyl-β-D-glucopyranoside (pNPG). The optimal temperature and pH for the enzymatic reaction of the histidine-tagged CMCase was 50 °C and 5.0. The histidine-tagged CMCase was enhanced by CoCl2 until the concentration of 100 mM, but inhibited by EDTA, HgCl2, MnCl2, NiCl2, and RbCl2. The characteristics of the histidine-tagged CMCase produced by E. coli BL21/A-53 were compared with those of CMCase without the histidine-tag of Bacillus subtilis subsp. subtilis A-53. The little changed characteristics of the histidine-tagged CMCase compared to the CMCase without a His-tag seemed to be the conformational change in the structure due to a His-tag. [ABSTRACT FROM AUTHOR]

Published

2019

31. An effective, simple and low-cost pretreatment for culture clarification in tetanus toxoid production.

Author

Avila, Lucía, Cascone, Osvaldo, Biscoglio, Mirtha, and Fingermann, Matías

Subjects

*TETANUS toxin, *TETANUS vaccines, *MICROFILTRATION, *EXTRAPOLATION, *CHITOSAN

Abstract

Chemically inactivated tetanus toxin (tetanus toxoid, TT), purified from cultures of a virulent Clostridium tetani strain, is the active pharmaceutical ingredient of anti-tetanus vaccines. Culture clarification for TT production and is usually performed by filtration-based techniques. Final clarification of the culture supernatant is achieved by passage through 0.2 µm pore size filtering membranes. Large particles removal (primary clarification) before final filtration (secondary clarification) reduces costs of the overall clarification process. With this aim, chitosan-induced particle aggregation was assessed as an alternative for primary clarification. Three chitosan variants were tested with similar results. Optimal clarification of culture supernatant was achieved by the addition of 8 mg chitosan per l of culture. Extrapolation analysis of filter sizing results indicate that 100 l of chitosan-treated supernatant can be finally filtered with a 0.6 m2 normal filtration cartridge of 0.45 + 0.2 µm pore size. The clarified material is compatible with current standard downstream processing techniques for TT purification. Thus, chitosan-induced particle aggregation is a suitable operation for primary clarification. [ABSTRACT FROM AUTHOR]

Published

2018

32. Optimization and purification of glucansucrase produced by Leuconostoc mesenteroides DRP2-19 isolated from Chinese Sauerkraut.

Author

Du, Renpeng, Zhao, Fangkun, Pan, Lei, Han, Ye, Xiao, Huazhi, and Zhou, Zhijiang

Subjects

*GLYCOSYLTRANSFERASES, *SAUERKRAUT, *LEUCONOSTOC mesenteroides, *SUCROSE, *FERMENTATION

Abstract

Strain DRP2-19 was detected to produce high yield of glucansucrase in MRS broth, which was identified to be Leuconostoc mesenteroides. In order for industrial glucansucrase production of L. mesenteroides DRP2-19, a one-factor test was conducted, then response surface method was applied to optimize its yield and discover the best production condition. Based on Plackett-Burman (PB) experiment, sucrose, Ca2+, and initial pH were found to be the most significant factors for glucansucrase production. Afterwards, effects of the three main factors on glucansucrase activity were further investigated by central composite design and the optimum composition was sucrose 35.87 g/L, Ca2+ 0.21 mmol/L, and initial pH 5.56. Optimum results showed that glucansucrase activity was increased to 3.94 ± 0.43 U/mL in 24 hr fermentation, 2.66-fold higher than before. In addition, the crude enzyme was purified using ammonium sulfate precipitation, ion-exchange chromatography, and gel filtration. The molecular weight of glucansucrase was determined as approximately 170 kDa by Sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE). The enzyme was purified 15.77-fold and showed a final specific activity of 338.56 U/mg protein. [ABSTRACT FROM AUTHOR]

Published

2018

33. Polyclonal antibody production against rGPC3 and their application in diagnosis of hepatocellular carcinoma.

Author

Wang, Shenghao, Kalim, Muhammad, Liang, Keying, and Zhan, Jinbiao

Subjects

*GLYPICANS, *LIVER cancer, *PROTEOGLYCANS, *CELL membranes, *GLYCOSYLPHOSPHATIDYLINOSITOL, *IMMUNOGLOBULINS, *LABORATORY rabbits

Abstract

Glypican-3 (GPC3) is an integral membrane proteoglycan, which contains a core protein anchored to the cytoplasmic membrane through a glycosylphosphatidylinositol linkage. The glypican-3 can regulate the signaling pathways, thereby enhances cell division, growth, and apoptosis in certain cell types. It is almost nonexistent on the surface of the human normal cell membrane and highly expresses on the membrane of hepatocellular carcinoma (HCC) cells. It has been well established that GPC3 provides a useful diagnostic marker. For generating the polyclonal antibody of GPC3, we expected that GPC3 N-terminal region (amino acid sequence 26-358) could be expressed in Escherichia coli system, however, no active expression was observed after IPTG induction. Interestingly, after deletion of six proline residues from position 26 to 31 in the N-terminus, expression of recombinant GPC3 was clearly detected. We further analyzed the expressed protein deprived of six prolines, to immunize the New Zealand male rabbits for production of active antibodies. The binding affinity of antibody was analyzed by immunofluorescence analysis, immunohistochemical detection, and western blotting. The functional GPC3 N-terminal protein recombinant development, expression, purification, and the polyclonal antibody have been generated provide the basis for the diagnosis of HCC in cancer therapy. [ABSTRACT FROM AUTHOR]

Published

2018

34. Expression, purification, crystallization, and diffraction analysis of a selenomethionyl lipase Lip8 from <italic>Yarrowia lipolytica</italic>.

Author

Jun, Sheng, XiaoFeng, Ji, Yuan, Zheng, and Mi, Sun

Subjects

*CRYSTALLIZATION, *DIFFRACTION patterns, *LIPASES, *ISOENZYMES, *PROTEIN expression

Abstract

Yarrowia lipolytica is a nonconventional model micro-organism with multiple biotechnological applications. It is also considered to be an excellent producer for lipase. Genome survey shows that Y. lipolytica possesses various paralogs of genes coding for extracellular, cell-bound, and intracellular lipolytic enzymes. However, little structural information on these isoenzymes is available. With the aim to facilitate crystal structure solution of Lip8, one of the most valuable lipases from Y. lipolytica, a less conventional protein expression technique—selenomethionyl protein expression was used to produce recombinant selenomethionine (SeMet)-Lip8 in Escherichia coli. Finally, three Met residues of Lip8 were all substituted with SeMet. A total of 72 mg of SeMet-Lip8 was obtained from a liter of the SeMet medium. Using sodium acetate as a precipitant and ammonium sulfate as an additive, crystals of the SeMet-Lip8 with 1.9 Å were successfully cultured through hanging-drop vapor diffusion method. The estimated crystal dimensions were 0.11 × 0.11 × 0.14 mm2. The crystal belonged to the space group I4 with unit cell parameters a = b = 128.87 Å, c = 171.77 Å, α = β = γ = 90°. It is the second member of lipase crystal family from Y. lipolytica. This work will provide a platform for further studying lipases from a structural insight. [ABSTRACT FROM AUTHOR]

Published

2018

35. Extraction, purification, and biochemical characterization of serine protease from leaves of Abrus precatorius.

Author

Serge, Ngangoum Eric, Laurette Blandine, Mezajoug Kenfack, Kumar, Sanjit, Clergé, Tchiégang, and Vijayalakshmi, Mookambeswaran

Subjects

*SERINE proteinases, *GEL permeation chromatography, *ION exchange chromatography, *MOLECULAR weights, *SODIUM dodecyl sulfate, *POLYACRYLAMIDE gel electrophoresis

Abstract

A protease from fresh leaves ofAbrus precatoriuswas purified using two classical chromatography techniques: ion-exchange (DEAE-Sepharose) and Gel filtration (Sephadex G-75). The purified protease showed a molecular weight of ∼ 28 kDa on sodium dodecyl sulfate polyacrylamide gel electrophoresis. The optimum pH and temperature for the purified protease was 8 and 40°C, respectively. The purified protease was stable throughout a wide temperature range from 10 to 80°C and pH from 2 to 12. Protease activity was inhibited in the presence of Co2+, Ni2+, Hg2+, and Zn2+while its activity has increased in the presence of Ca2+and Mg2+. The protease was highly specific to casein when compared to its specificity for gelatin, bovine serum albumin, hemoglobin, and defatted flour ofRicinodendron heudelotii.ItsVmaxandKmdetermined using casein as a substrate were 94.34 U/mL and 349.07 µg/mL respectively. Inhibition studies showed that this purified protease was inhibited by both phenylmethane sulfonyl fluoride and aprotinin which are recognized as competitive inhibitors of serine proteases. [ABSTRACT FROM AUTHOR]

Published

2017

36. Aqueous two-phase assisted by ultrasound for the extraction of anthocyanins from Lycium ruthenicum Murr.

Author

Qin, Benlin, Liu, Xuecong, Cui, Haiming, Ma, Yue, Wang, Zimin, and Han, Jing

Subjects

*ANTHOCYANINS, *TWO-phase flow, *ETHANOL, *EXTRACTION (Chemistry), *BIOACTIVE compounds

Abstract

In this study, an efficient ultrasound-assisted aqueous two-phase extraction method was used for the extraction of anthocyanins fromLycium ruthenicumMurr. An ethanol/ammonium sulfate system was chosen for the aqueous two-phase system due to its fine partitioning and recycling behaviors. Single-factor experiments were conducted to determine the optimized composition of the system, and the response surface methodology was used for the further optimization of the ultrasound-assisted aqueous two-phase extraction. The optimal conditions were as follows: a salt concentration of 20%, an ethanol concentration of 25%, an extraction time of 33.7 min, an extraction temperature of 25°C, a liquid/solid ratio of 50:1 w/w, pH value of 3.98, and an ultrasound power of 600 W. Under the above conditions, the yields of anthocyanins reached 4.71 mg/g dry sample. For the further purification, D-101 resin was used, and the purity of anthocyanins reached 25.3%. In conclusion, ultrasound-assisted aqueous two-phase extraction was an efficient, ecofriendly, and economical method, and it may be a promising technique for extracting bioactive components from plants. [ABSTRACT FROM PUBLISHER]

Published

2017

37. Purification of antibody against Ara h 2 by a homemade immunoaffinity chromatography column.

Author

Wu, Zhihua, Li, Kun, Zhan, Shaode, Tong, Ping, Li, Xin, Yang, Anshu, and Chen, Hongbing

Subjects

*IMMUNOAFFINITY chromatography, *IMMUNOGLOBULINS, *AGAROSE, *BLOOD proteins, *IMMUNE serums

Abstract

Antibodies are used extensively in numerous applications bothin vivoandin vitro. To purify anti-Ara h 2 polyclonal antibody, a homemade immunoaffinity chromatography (IAC) column method was established. The properties of homemade column were compared with those of the mAb affinity protein G (MPG) agarose high flow, a commercially available column successfully used in capturing polyclonal antibodies. During antibody purification from rabbits’ antiserum against Ara h 2, the column capacity, recovery, and purification factor were characterized for IAC and MPG. The homemade IAC could separate the corresponding antibody with higher specificity and lower cost but with lower recovery and column capacity than those of MPG. Thus, the homemade IAC is a specific, inexpensive, and suitable method that can be used for various laboratory purifications. [ABSTRACT FROM PUBLISHER]

Published

2017

38. High-yield of biologically active recombinant human fibroblast growth factor-16 in E. coli and its mechanism of proliferation in NCL-H460 cells.

Author

Cheng, Jiliang, Fang, Zhaoxiang, Yang, Huanhuan, Li, Yong, Tian, Haishan, Gong, Weiyue, Chen, Taotao, Liu, Min, Li, Xiaokun, and Jiang, Chao

Subjects

*FIBROBLAST growth factors, *BIOACTIVE compounds, *ESCHERICHIA coli, *CANCER cell proliferation, *MITOSIS, *TUMOR growth, *CANCER invasiveness

Abstract

Fibroblast growth factor-16 (FGF16) is a member of FGF9 subfamily, which plays key role in promoting mitosis and cell survival, and also involved in embryonic development, cell growth, tissue repair, morphogenesis, tumor growth, and invasion. However, the successful high-yield purification of recombinant human fibroblast growth factor-16 (rhFGF16) protein has not been reported. In addition, lung cancer is a major cause of cancer-related deaths, which threats people’s lives and its incidence has continued to rise. Learning pathways or proteins, which involved in lung tumor progression will contribute to the development of early diagnosis and targeted therapy. FGF16 promoted proliferation and invasion behavior of SKOV-3 ovarian cancer cells, whose function may be similar in lung cancer. The hFGF16 was cloned into pET-3d and expressed inEscherichia coliBL21 (DE3) pLysS. Finally, obtained two forms of FGF16 that exhibited remarkable biological activity and the purity is over 95%, meanwhile, the yield of soluble 130 mg/100 g and insoluble 240 mg/100 g. Experiments demonstrated FGF16 could promote proliferation of NCL-H460 cells by activating Akt, Erk1/2, and p38 MAPK signaling, whereas JNK had no significant effect. In total, this optimized expression strategy enables significant quantity and activity of rhFGF16, thereby meeting its further pharmacological and clinical usages. [ABSTRACT FROM AUTHOR]

Published

2017

39. Production of a protease inhibitor from edible mushroom Agaricus bisporus and its statistical optimization by response surface methodology.

Author

Vishvakarma, Reena and Mishra, Abha

Subjects

*CULTIVATED mushroom, *EDIBLE mushrooms, *PROTEASE inhibitors, *SOLID-state fermentation, *MATHEMATICAL optimization, *RESPONSE surfaces (Statistics)

Abstract

The production of a protease inhibitor fromAgaricus bisporusthrough solid-state fermentation was studied. The purpose was to produce protease inhibitor from natural, cheap, and readily available carbon and nitrogen sources. Solid-state fermentation enhanced the mycelia growth and also gave a higher yield of the product. Further, fungal growth and other production parameters were statistically optimized. The specificity of the inhibitor was tested and was effective against trypsin. Screening of significant factors (wheat bran, cyanobacterial biomass, initial pH, temperature, incubation period, and moisture content and inoculum size) was performed using Plackett–Burman design. Central composite design was used to determine the optimized values of the significant variables which were found to be temperature (27.5°C), incubation time (156 hr), cyanobacterial biomass (1 g), and moisture content (50%) and gave a statistical yield of 980 PIU/g which was 25.6% higher than experimental yield (780 PIU/g). The inhibitor was purified by ammonium sulfate precipitation and diethylaminoethyl (DEAE) cellulose chromatography (yield 43.89% and 0.21%, respectively) and subjected to reversed-phase HPLC to validate its identity. Since protease inhibitors act against proteases, finding ample therapeutic roles; the isolated protease inhibitor fromA. bisporuscan also be a probable medicinal agent after its further characterization. [ABSTRACT FROM PUBLISHER]

Published

2017

40. Purification and characterization of a novel trypsin-like protease from green-seeded chickpea ( Cicer arientum ).

Author

Shamsi, Tooba Naz, Parveen, Romana, Sen, Priyankar, and Fatima, Sadaf

Subjects

*CHICKPEA, *TRYPSIN, *ENZYMES, *FOOD, *ION exchange (Chemistry), *CHROMATOGRAPHIC analysis, *PROTEOLYTIC enzymes, *AMMONIUM sulfate

Abstract

The present study describes the purification and physicochemical and biochemical characterization of trypsin-like protease from green-seeded chickpea (Cicer arientum). The crude extract of chickpea trypsin (CpT) was obtained by homogenization followed by differential ammonium sulfate precipitation. The CpT was purified by ion-exchange chromatography on diethylaminoethyl (DEAE) column, pre-equilibrated with 20 mM tris-CaCl2buffer (pH 8.2) with a flow rate of 0.5 mL min−1. The molecular weight and purity of ∼23 kDa of CpT were determined by sodium dodecyl sulfate polyacrylamide gel electrophoresis. Activity of protease was determined usingNα-benzoyl-DL-arginine-p-nitroanilide as chromogenic substrate and CpT purified showed a specific inhibitor activity of 26978.7697 U mg−1, fold purity of 9.8, and the yield of 70.2%. The characterization was performed for thermal stability, pH profile, and effect of various inhibitors on enzymatic activity. The protein isolated showed stability in the neutral to mild alkaline pH range and thermostability up to 50°C. CpT confirmed its serine nature as it was appreciably inhibited by serine protease inhibitors (maximum 6%), whereas metalloprotease inhibitors barely affected the activity of the enzyme (85%). To the best of our knowledge, it is first reported on purification of protease with trypsin-like properties, from this source. [ABSTRACT FROM PUBLISHER]

Published

2017

41. Isolation, purification, and partial characterization of a membrane-bound Cl /HCO 3 -activated ATPase complex from rat brain with sensitivity to GABA A ergic ligands.

Author

Menzikov, Sergey A.

Subjects

*ADENOSINE triphosphatase, *GABA, *COORDINATION compounds, *RATS, *BRAIN

Abstract

This study describes the isolation and purification of a protein complex with-ATPase activity and sensitivity to GABAAergic ligands from rat brain plasma membranes. The ATPase complex was enriched using size-exclusion, affinity, and ion-exchange chromatography. The fractions obtained at each purification step were subjected to SDS-polyacrylamide gel electrophoresis (SDS-PAGE), which revealed four subunits with molecular mass ∼48, 52, 56, and 59 kDa; these were retained at all stages of the purification process. Autoradiography revealed that the ∼52 and 56 kDa subunits could bind [3H]muscimol. The-ATPase activity of this enriched protein complex was regulated by GABAAergic ligands but was not sensitive to blockers of the NKCC or KCC cotransporters. [ABSTRACT FROM PUBLISHER]

Published

2017

42. Heterologous expression and purification of neurotoxic Hainantoxin-III in E. coli.

Author

Wu, Hui, Chen, Bo, Jiang, Hui, Wu, Lei, Zhu, Ling-Yun, Meng, Er, and Zhang, Dong-Yi

Subjects

*NEUROTOXIC agents, *ESCHERICHIA coli, *AMINO acids, *SODIUM channels, *ULTRAFILTRATION

Abstract

In the present study, we usedEscherichia colito produce recombinant Hainantoxin-III (rHNTX-III), a 33-amino acid peptic toxin from the tarantula spiderHaplopelma hainanum. The toxin has three pairs of disulfide bonds. A pET-HS-HNTX-III vector was constructed and transformed into theE. colistrain SHuffleTM. rHNTX-III was expressed using auto-induction medium. After using a Ni–NTA column, the expressed fusion protein was digested using SUMO protease (ULP1) to remove the HIS–SUMO tag, and then RP–HPLC and ultrafiltration were used for further purification. Then the rHNTX-III was identified by MALDI–TOF/TOF mass spectrometry. The purified rHNTX-III was further analyzed using a whole-cell patch-clamp assay. It was shown that the rHNTX-III was able to block currents generated by human Nav1.7 (hNav1.7) at an IC50of 225 nM and also have high selectivity for different voltage-gated sodium channels. Therefore, it has very similar activity to the natural one. [ABSTRACT FROM PUBLISHER]

Published

2017

43. Gram-scale production of plasmid pUDK-HGF with current good manufacturing practices for gene therapy of critical limb ischemia.

Author

Hu, ChunSheng, Cheng, XiaoChen, Lu, YuXin, Wu, ZuZe, and Zhang, QingLin

Subjects

*PLASMIDS, *GENE therapy, *ISCHEMIA, *SEPHAROSE, *CHROMATOGRAPHIC analysis

Abstract

The demand of a plasmid encoding human hepatocyte growth factor gene (pUDK-HGF) in large quantities at high purity and concentration has increased for gene therapy of critical limb ischemia (CLI) in clinical trials. In this article, we produced pUDK-HGF in compliance with current good manufacturing practices at gram scale. The process included a 50-L batch fermentation, continuous alkaline lysis, and integrated three-step chromatography on Sepharose 6 Fast Flow, PlasmidSelect Xtra, and Source 15Q. The production process has been scaled up to yield 4.24 ± 0.41 g of pharmaceutical pUDK-HGF from 1.0 kg bacterial cell paste and the overall yield reached range from 58.37 to 66.70%. The final pUDK-HGF product exhibited high purity with supercoiled percentage of > 95.8% and undetectable residual RNA, contaminated protein, and bacterial endotoxin. The phase I clinical study indicates that intramuscular injection of pUDK-HGF is safe, well tolerated, and may provide symptomatic relief to CLI patients. These results show that our manufacturing process of pUDK-HGF is efficient in producing pharmaceutical-grade plasmid DNA and is safe for clinical applications. [ABSTRACT FROM AUTHOR]

Published

2016

44. Expression, purification, and characterization of recombinant human H-chain ferritin.

Author

Zou, Wenyan, Liu, Xiaoyu, Chen, Dianhua, Wang, Jie, Zhao, Xi, Li, Jiahuang, Ji, Lina, and Hua, Zichun

Subjects

*GENE expression, *RECOMBINANT antibodies, *FERRITIN genetics, *ESCHERICHIA coli, *BACTERIAL genetics, *SOLUBILITY

Abstract

Based on their nanocage architectures, ferritins show their potential applications in medical imaging and therapeutic delivery systems. However, the recombinant human H-chain ferritin (rHF) is prone to form inclusion bodies inEscherichia coli. In our study, the cDNA of rHF was cloned into plasmid pET28a under the control of a T7 promoter. Molecular chaperones, including GroES, GroEL, and trigger factor, were coexpressed with rHF to facilitate its correct folding. The results showed that the solubility of rHF was increased more than threefold with the help of molecular chaperones. Taking advantages of its N-terminal His-tag, rHF was then purified with Ni-affinity chromatography. With a yield of 15 mg/L from bacterial culture, the purified rHF was analyzed by circular dichroism spectrometry for its secondary structure. Moreover, the rHF nanocages were characterized by transmission electron microscopy and dynamic light scattering. Our results indicate that rHF is able to self-assemble into nanocages with a narrow size distribution. [ABSTRACT FROM AUTHOR]

Published

2016

45. Purification and characterization of a soluble glycoprotein from garlic ( Allium sativum ) and its in vitro bioactivity.

Author

Wang, Yan, Zou, Tingting, Xiang, Minghui, Jin, Chenzhong, Zhang, Xuejiao, Chen, Yong, Jiang, Qiuqing, and Hu, Yihong

Subjects

*GARLIC, *GLYCOPROTEINS, *FOURIER transform infrared spectroscopy, *HYDROLYSIS, *PEROXIDATION, *THERAPEUTICS

Abstract

A soluble glycoprotein was purified to homogeneity from ripe garlic (Allium sativum) bulbs using ammonium sulfate precipitation, Sephadex G-100 gel filtration, and diethylaminoethyl-52 cellulose anion-exchange chromatography. A native mass of 55.7 kDa estimated on gel permeation chromatography and a molecular weight of 13.2 kDa observed on sodium dodecyl sulfate-polyacrylamide gel electrophoresis supported that the glycoprotein is a homotetramer.β-Elimination reaction result suggested that the glycoprotein is anN-linked type. Fourier-transform infrared spectroscopy proved that it contains sugar. Gas chromatography–mass spectrometer analysis showed that its sugar component was galactose. The glycoprotein has 1,1-diphenyl-2-picrylhydrazil free radical scavenging activity and the peroxidation inhibition ability to polyunsaturated fatty acid. These results indicated that the glycoprotein has potential for food additives, functional foods, and even biotechnological and medical applications. [ABSTRACT FROM PUBLISHER]

Published

2016

46. Catalase purification from rat liver with iron-chelated poly(hydroxyethyl methacrylate- N -methacryloyl-( l )-glutamic acid) cryogel discs.

Author

Göktürk, Ilgım, Perçin, Işık, and Denizli, Adil

Subjects

*GLUTAMIC acid, *ADSORPTION (Chemistry), *LABORATORY rats, *CATALASE, *ENZYMES

Abstract

In this study, iron-chelated poly(hydroxyethyl methacrylate-N-methacryloyl-(l)-glutamic acid) (PHEMAGA/Fe3+) cryogel discs were prepared. The PHEMAGA/Fe3+ cryogel discs were characterized by elemental analysis, scanning electron microscopy, Fourier transform infrared spectroscopy, swelling tests, and surface area measurements. The PHEMAGA/Fe3+ cryogel discs had large pores ranging from 10 to 100 µm with a swelling degree of 9.36 g H2O/g cryogel. Effects of pH, temperature, initial catalase concentration, and flow rate on adsorption capacity of the PHEMAGA/Fe3+ cryogel discs were investigated. Maximum catalase adsorption capacity (62.6 mg/g) was obtained at pH 7.0, 25°C, and 3 mg/ml initial catalase concentration. The PHEMAGA/Fe3+ cryogel discs were also tested for the purification of catalase from rat liver. After tissue homogenization, purification of catalase was performed using the PHEMAGA/Fe3+ cryogel discs and catalase was obtained with a yield of 54.34 and 16.67 purification fold. [ABSTRACT FROM AUTHOR]

Published

2016

47. A method for efficient expression of Pseudomonas aeruginosa alginate lyase in Pichia pastoris.

Author

Yue, Michael M., Gong, Wendy W., Qiao, Yu, and Ding, Hongbiao

Subjects

*PICHIA pastoris, *ALGINATE lyase, *PSEUDOMONAS aeruginosa, *FUNGAL gene expression, *RECOMBINANT proteins, *KANAMYCIN, *AMPICILLIN

Abstract

As an eco-friendly biocatalyst for alginate hydrolysis, bacteria-derived alginate lyase (AlgL) has been widely used in research and industries to produce oligosaccharides. However, the cost of AlgL enzyme production remains high due to the low expression and difficulty in purification from bacterial cells. In this study we report an effective method to overexpress thePseudomonas aeruginosaAlgL (paAlgL) enzyme inPichia pastoris. Fused with a secretory peptide, the recombinant paAlgL was expressed extracellularly and purified from the culture supernatant through a simple process. The purified recombinant enzyme is highly specific for alginate sodium with a maximal activity of 2,440 U/mg. The enzymatic activity remained stable below 45°C and at pH between 4 and 10. The recombinant paAlgL was inhibited by Zn2+, Cu2+, and Fe2+and promoted by Co2+and Ca2+. Interestingly, we also found that the recombinant paAlgL significantly enhanced the antimicrobial activity of antibiotics ampicillin and kanamycin againstPseudomonas aeruginosa. Our results introduce a method for efficient AlgL production, the characterization, and a new feature of the recombinant paAlgL as an enhancer of antibiotics againstPseudomonas aeruginosa. [ABSTRACT FROM PUBLISHER]

Published

2016

48. Purification of anti-bromelain antibodies by affinity precipitation using pNIPAm-linked bromelain.

Author

Mahmood, Rubab

Subjects

*IMMUNOGLOBULIN analysis, *BROMELIN, *PRECIPITATION (Chemistry), *ACRYLAMIDE derivatives, *ENZYME-linked immunosorbent assay, *PROTEIN fractionation, *AFFINITY electrophoresis

Abstract

Affinity precipitation has emerged as a very useful technique for the purification of proteins. Here it has been employed for the purification of anti-bromelain antibodies from rabbit serum. A system has been developed for reversibly binding and thermoprecipitating antibodies. Anti-bromelain antibodies were raised in rabbit by immunizing it with bromelain. Poly-N-isopropylacrylamide (pNIPAm)–bromelain conjugate was prepared and incubated with rabbit serum. After that the temperature was raised for thermal precipitation of the polymer. Antibodies were then eluted from the complex by incubating it with a small volume of buffer, pH 3.0. This method is very effective in concentrating the antibodies. Purity and specificity of the antibodies were checked by gel electrophoresis and enzyme-linked immunosorbent assay (ELISA), respectively. The study of the effect of pH and temperature on the binding of the antibodies to the conjugate showed that the optimum binding occurred at pH 8.0 and 25°C.The polymer enzyme conjugate was further used for another cycle. [ABSTRACT FROM PUBLISHER]

Published

2016

49. Expression and purification of the recombinant porcine NK-lysin in Pichia pastoris and observation of anticancer activity in vitro.

Author

Fan, Kuohai, Li, Hongquan, Wang, Zhirui, Du, Wenjuan, Yin, Wei, Sun, Yaogui, and Jiang, Junbing

Subjects

*KILLER cells, *CELL lines, *SACCHAROMYCETACEAE, *ERYTHROCYTES, *HEMOLYSIS & hemolysins

Abstract

Natural killer (NK)-lysin, a broad-spectrum antimicrobial peptide, has antitumor and antibactericidal activities against both gram-positive and gram-negative bacteria. In this study the recombinant porcine NK-lysin was expressed and purified in thePichia pastorissystem, and then 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide was used to assess its anticancer activityin vitro. The results showed that the recombinant porcine NK-lysin possesses potent antitumor activity against the human hepatocellular carcinoma cell line SMMC-7721 in a time- and dose-dependent manner, but has negligible hemolysis activity against human erythrocytes. Scanning electronic microscopy was used to directly observe the ultrastructure of SMMC-7721 cells treated with NK-lysin; untreated cells showed lamellipodia and filopodia scattered with the cell surface, with good cell–cell contacts among neighboring cells. In contrast, treated tumor cells exhibited marked alterations in cell morphology, and cell–cell contacts disappeared among neighboring cells. Compared with the untreated tumor cells, the tumor cells treated with NK-lysin for 12 and 24 hr were suppressed for the expression of fascin 1. Thus, the recombinant porcine NK-lysin potentially could be developed as a therapeutic agent for inhibiting tumor growth. [ABSTRACT FROM AUTHOR]

Published

2016

50. Optimization, purification, and characterization of L-asparaginase from Actinomycetales bacterium BkSoiiA.

Author

Dash, Chitrangada, Mohapatra, Sukanti Bala, and Maiti, Prasanta Kumar

Subjects

*ACTINOBACTERIA, *ASPARAGINASE, *GLYCOASPARAGINASE, *ACTINOMYCETALES, *BACTERIA

Abstract

Actinobacteria are promising source of a wide range of important enzymes, some of which are produced in industrial scale, with others yet to be harnessed. L-Asparaginase is used as an antineoplastic agent. The present work deals with the production and optimization of L-asparaginase fromActinomycetales bacteriumBkSoiiA using submerged fermentation in M9 medium. Production optimization resulted in a modified M9 medium with yeast extract and fructose as carbon and nitrogen sources, respectively, at pH 8.0, incubated for 120 hr at 30 ± 2°C. The crude enzyme was purified to near homogeneity by ammonium sulfate precipitation following dialysis, ion-exchange column chromatography, and finally gel filtration. The sodium dodecyl sulfate (SDS) polyacrylamide gel electrophoresis (PAGE) revealed an apparent molecular weight of 57 kD. The enzyme was purified 95.06-fold and showed a final specific activity of 204.37 U/mg with 3.49% yield. The purified enzyme showed maximum activity at a pH 10.0 and was stable at pH 7.0 to 9.0. The enzyme was activated by Mn2+and strongly inhibited by Ba2+. All these preliminary characterization suggests that the L-asparaginase from the source may be a tool useful to pharmaceutical industries after further research. [ABSTRACT FROM AUTHOR]

Published

2016