Resumo
Instead of typical household trash, the heavy metal complexes, organic chemicals, and other poisons produced by huge enterprises threaten water systems across the world. In order to protect our drinking water from pollution, we must keep a close eye on the situation. Nanotechnology, specifically two-dimensional (2D) nanomaterials, is used in certain wastewater treatment systems. Graphene, g-C3N4, MoS2, and MXene are just a few examples of emerging 2D nanomaterials that exhibit an extraordinary ratio of surface (m3), providing material consumption, time consumption, and treatment technique for cleaning and observing water. In this post, we'll talk about the ways in which 2D nanomaterials may be tuned to perform certain functions, namely how they can be used for water management. The following is a quick overview of nanostructured materials and its possible use in water management: Also discussed in length are the applications of 2D nanomaterials in water purification, including pollutant adsorption, filtration, disinfection, and photocatalysis. Fluorescence sensors, colorimetric, electrochemical, and field-effect transistors are only some of the devices being studied for their potential use in monitoring water quality using 2D nanomaterials. Utilizing 2D content has its benefits and pitfalls when used to water management. New developments in this fast-expanding business will boost water treatment quality and accessibility in response to rising awareness of the need of clean, fresh water among future generations.
Em vez do lixo doméstico típico, os complexos de metais pesados, produtos químicos orgânicos e outros venenos produzidos por grandes empresas ameaçam os sistemas de água em todo o mundo. Para proteger nossa água potável da poluição, devemos ficar de olho na situação. A nanotecnologia, especificamente nanomateriais bidimensionais (2D), é usada em certos sistemas de tratamento de águas residuais. Grafeno, g-C3N4, MoS2 e MXene são apenas alguns exemplos de nanomateriais 2D emergentes que exibem uma extraordinária proporção de superfície (m3), proporcionando consumo de material, consumo de tempo e técnica de tratamento para limpeza e observação da água. Neste trabalho, trataremos das maneiras pelas quais os nanomateriais 2D podem ser ajustados para desempenhar determinadas funções, ou seja, como eles podem ser usados para o gerenciamento de água. A seguir, uma breve visão geral dos materiais nanoestruturados e seu possível uso no gerenciamento de água. Serão também discutidas detalhadamente as aplicações de nanomateriais 2D na purificação de água, incluindo adsorção de poluentes, filtração, desinfecção e fotocatálise. Sensores de fluorescência, colorimétricos, eletroquímicos e transistores de efeito de campo são apenas alguns dos dispositivos que estão sendo estudados para uso potencial no monitoramento da qualidade da água usando nanomateriais 2D. A utilização de conteúdo 2D tem seus benefícios e armadilhas quando utilizada para gerenciamento de água. Novos desenvolvimentos neste negócio em rápida expansão visam aumentar a qualidade e a acessibilidade do tratamento de água em resposta à crescente conscientização sobre a necessidade de água limpa e fresca entre as gerações futuras.
Assuntos
Poluição da Água/prevenção & controle , Monitoramento da Água , Purificação da Água , NanoestruturasResumo
The production of antivenom from immunized animals is an established treatment for snakebites; however, antibody phage display technology may have the capacity to delivery results more quickly and with a better match to local need. Naja oxiana, the Iranian cobra, is a medically important species, responsible for a significant number of deaths annually. This study was designed as proof of principle to determine whether recombinant antibodies with the capacity to neutralize cobra venom could be isolated by phage display. Methods: Toxic fractions from cobra venom were prepared by chromatography and used as targets in phage display to isolate recombinant antibodies from a human scFv library. Candidate antibodies were expressed in E. coli HB2151 and purified by IMAC chromatography. The selected clones were analyzed in in vivo and in vitro experiments. Results: Venom toxicity was contained in two fractions. Around a hundred phage clones were isolated against each fraction, those showing the best promise were G12F3 and G1F4. While all chosen clones showed low but detectable neutralizing effect against Naja oxiana venom, clone G12F3 could inhibit PLA2 activity. Conclusion: Therefore, phage display is believed to have a good potential as an approach to the development of snake antivenom.(AU)
Assuntos
Animais , Mordeduras de Serpentes , Bacteriófagos/isolamento & purificação , Antivenenos , Venenos Elapídicos/síntese química , Anticorpos , Técnicas In VitroResumo
Background:The production of antivenom from immunized animals is an established treatment for snakebites; however, antibody phage display technology may have the capacity to delivery results more quickly and with a better match to local need. Naja oxiana, the Iranian cobra, is a medically important species, responsible for a significant number of deaths annually. This study was designed as proof of principle to determine whether recombinant antibodies with the capacity to neutralize cobra venom could be isolated by phage display.Methods:Toxic fractions from cobra venom were prepared by chromatography and used as targets in phage display to isolate recombinant antibodies from a human scFv library. Candidate antibodies were expressed in E. coli HB2151 and purified by IMAC chromatography. The selected clones were analyzed in in vivo and in vitro experiments.Results:Venom toxicity was contained in two fractions. Around a hundred phage clones were isolated against each fraction, those showing the best promise were G12F3 and G1F4. While all chosen clones showed low but detectable neutralizing effect against Naja oxiana venom, clone G12F3 could inhibit PLA2 activity.Conclusion:Therefore, phage display is believed to have a good potential as an approach to the development of snake antivenom.(AU)
Assuntos
Animais , Naja naja , Venenos Elapídicos/antagonistas & inibidores , Antivenenos/análise , Terapia por Fagos , ColífagosResumo
Beta-cardiotoxin (ß-CTX), the three-finger toxin isolated from king cobra (Ophiophagus hannah) venom, possesses ß-blocker activity as indicated by its negative chronotropy and its binding property to both ß-1 and ß-2 adrenergic receptors and has been proposed as a novel ß-blocker candidate. Previously, ß-CTX was isolated and purified by FPLC. Here, we present an alternative method to purify this toxin. In addition, we tested its cytotoxicity against different mammalian muscle cell types and determined the impact on cardiac function in isolated cardiac myocyte so as to provide insights into the pharmacological action of this protein. Methods: ß-CTX was isolated from the crude venom of the Thai king cobra using reverse-phased and cation exchange HPLC. In vitro cellular viability MTT assays were performed on mouse myoblast (C2C12), rat smooth muscle (A7r5), and rat cardiac myoblast (H9c2) cells. Cell shortening and calcium transient dynamics were recorded on isolated rat cardiac myocytes over a range of ß-CTX concentration. Results: Purified ß-CTX was recovered from crude venom (0.53% w/w). MTT assays revealed 50% cytotoxicity on A7r5 cells at 9.41 ± 1.14 µM (n = 3), but no cytotoxicity on C2C12 and H9c2 cells up to 114.09 µM. ß-CTX suppressed the extend of rat cardiac cell shortening in a dose-dependent manner; the half-maximal inhibition concentration was 95.97 ± 50.10 nM (n = 3). In addition, the rates of cell shortening and re-lengthening were decreased in ß-CTX treated myocytes concomitant with a prolongation of the intracellular calcium transient decay, indicating depression of cardiac contractility secondary to altered cardiac calcium homeostasis. Conclusion: We present an alternative purification method for ß-CTX from king cobra venom. We reveal cytotoxicity towards smooth muscle and depression of cardiac contractility by this protein. These data are useful to aid future development of pharmacological agents derived from ß-CTX.(AU)
Assuntos
Animais , Charibdotoxina/isolamento & purificação , Miócitos Cardíacos , Proteínas Cardiotóxicas de Elapídeos , Venenos Elapídicos , Cardiotoxinas , Ophiophagus hannah , Supressão , Citotoxicidade ImunológicaResumo
Beta-cardiotoxin (ß-CTX), the three-finger toxin isolated from king cobra (Ophiophagus hannah) venom, possesses ß-blocker activity as indicated by its negative chronotropy and its binding property to both ß-1 and ß-2 adrenergic receptors and has been proposed as a novel ß-blocker candidate. Previously, ß-CTX was isolated and purified by FPLC. Here, we present an alternative method to purify this toxin. In addition, we tested its cytotoxicity against different mammalian muscle cell types and determined the impact on cardiac function in isolated cardiac myocyte so as to provide insights into the pharmacological action of this protein. Methods: ß-CTX was isolated from the crude venom of the Thai king cobra using reverse-phased and cation exchange HPLC. In vitro cellular viability MTT assays were performed on mouse myoblast (C2C12), rat smooth muscle (A7r5), and rat cardiac myoblast (H9c2) cells. Cell shortening and calcium transient dynamics were recorded on isolated rat cardiac myocytes over a range of ß-CTX concentration. Results: Purified ß-CTX was recovered from crude venom (0.53% w/w). MTT assays revealed 50% cytotoxicity on A7r5 cells at 9.41 ± 1.14 µM (n = 3), but no cytotoxicity on C2C12 and H9c2 cells up to 114.09 µM. ß-CTX suppressed the extend of rat cardiac cell shortening in a dose-dependent manner; the half-maximal inhibition concentration was 95.97 ± 50.10 nM (n = 3). In addition, the rates of cell shortening and re-lengthening were decreased in ß-CTX treated myocytes concomitant with a prolongation of the intracellular calcium transient decay, indicating depression of cardiac contractility secondary to altered cardiac calcium homeostasis. Conclusion: We present an alternative purification method for ß-CTX from king cobra venom. We reveal cytotoxicity towards smooth muscle and depression of cardiac contractility by this protein. These data are useful to aid future development of pharmacological agents derived from ß-CTX.(AU)
Assuntos
Animais , Venenos Elapídicos/análise , Venenos Elapídicos/isolamento & purificação , Miócitos Cardíacos/fisiologia , Cardiotoxinas/administração & dosagemResumo
Septin14 is an important spermatogenesis related gene involved in the pathogenesis of male infertility that has not been well studied. Here, full-length Septin14 cDNA of the Banna mini-pig inbred line (BMI) was cloned using the RACE method and expressed in pig kidney epithelial cells (PK15) and E. coli Rosetta (DE3) cells. Septin14 expression was identified in somatic tissues and testis in different developmental stages. The pig Septin14 CDS is 1,299 bp long, and encodes a peptide (or protein) of 432 amino acids (MW=50.4 kDa). Phylogenetic analysis indicated that pig Septin14 was highly evolutionarily conserved. Subcellular localization of GFP-tagged Septin14 fusion protein revealed that Septin14 was distributed throughout the testicular cells. Among 34 pig tissues, Septin14 mRNA was found specifically in testis and seminal vesicle. In six different postnatal developmental stages, the testicular level of Septin14 mRNA was barely detectable on day 2, while the highest level occurred on day 75. The spatiotemporal expression profile of Septin14, reported herein for the first time in pig, indicated that Septin14 might be involved in the division, development and apoptosis of germ cells. Furthermore, using a pET prokaryotic expression system, we expressed and isolated recombinant 67.9 kDa Septin14 protein.
Assuntos
Masculino , Animais , Clonagem Molecular , Glândulas Seminais , Septinas/análise , Septinas/classificação , Suínos/fisiologia , Suínos/genéticaResumo
Septin14 is an important spermatogenesis related gene involved in the pathogenesis of male infertility that has not been well studied. Here, full-length Septin14 cDNA of the Banna mini-pig inbred line (BMI) was cloned using the RACE method and expressed in pig kidney epithelial cells (PK15) and E. coli Rosetta (DE3) cells. Septin14 expression was identified in somatic tissues and testis in different developmental stages. The pig Septin14 CDS is 1,299 bp long, and encodes a peptide (or protein) of 432 amino acids (MW=50.4 kDa). Phylogenetic analysis indicated that pig Septin14 was highly evolutionarily conserved. Subcellular localization of GFP-tagged Septin14 fusion protein revealed that Septin14 was distributed throughout the testicular cells. Among 34 pig tissues, Septin14 mRNA was found specifically in testis and seminal vesicle. In six different postnatal developmental stages, the testicular level of Septin14 mRNA was barely detectable on day 2, while the highest level occurred on day 75. The spatiotemporal expression profile of Septin14, reported herein for the first time in pig, indicated that Septin14 might be involved in the division, development and apoptosis of germ cells. Furthermore, using a pET prokaryotic expression system, we expressed and isolated recombinant 67.9 kDa Septin14 protein.(AU)
Assuntos
Animais , Masculino , Suínos/genética , Suínos/fisiologia , Septinas/análise , Septinas/classificação , Glândulas Seminais , Clonagem MolecularResumo
Techniques to decrease losses from bacterial diseases are always important to improve the fish production. The use of antagonistic substances (bacteriocins) has been proven to be a viable option. The aim of this study was to evaluate different methods of purification for bacteriocin like inhibitory substances (BLIS). For the purification process, we isolated and used two Gram-positive bacilli that produce antagonistic substances for pathogens in aquaculture. Tests for detection of interfering factors were also performed. After the confirmation that the antagonistic action was due the BLIS activity, we carried out the purification methods. The methods tested were: cell free supernatant, acid extraction and ammonium sulfate precipitation at two concentrations (20 and 50%). Salmonella Tiphy CFP/IAL1472 and Aeromonas hydrophila (isolated in a tilapia production environment) were used as indicators of the efficiency of extracts in controlling pathogenic potentials. Ammonium sulfate precipitation at 50% was the most appropriate for purifying the antagonistic substance for both indicators. The extracts of the two isolates remained active for 22 days at 25ºC. These are promising results regarding the water and fish health without the use of antibiotics, in this manner being a safer environmental practice.
Técnicas para diminuir as perdas causadas por doenças bacterianas são importantes para melhorar continuamente a produção de pescado. O uso de substâncias antagônicas (bacteriocinas) tem-se mostrado uma opção viável. O objetivo do trabalho foi avaliar diferentes métodos de purificação de bacteriocinas como substâncias inibidoras (BLIS). Dois bacilos Gram-positivos, produtores de substâncias antagonistas para agentes patogênicos da aquicultura, foram utilizados em processos de purificação. Depois de confirmada a ação antagônica pela atividade de BLIS, os métodos de purificação foram realizados. Os métodos testados foram: células livres de sobrenadante, extração ácida e precipitação por sulfato de amônia em duas concentrações (20 e 50%). Salmonella Typhi PCP/IAL1472 e Aeromonas hydrophila (isolada de um ambiente de tilapicultura) foram utilizadas como indicadores de eficiência dos extratos. O precipitado por sulfato de amônio a 50% foi o mais adequado para purificar a substância antagonista para ambos os isolados indicadores. Os extratos dos dois isolados permaneceram ativos por 22 dias em 25ºC. Estes resultados são promissores do ponto de vista da manutenção da sanidade da água e dos peixes, sem uso de antibióticos, constituindo uma prática ambientalmente mais segura.
Assuntos
Bacilos Gram-Positivos/isolamento & purificação , Bacteriocinas/isolamento & purificação , Pesqueiros/análise , AquiculturaResumo
Techniques to decrease losses from bacterial diseases are always important to improve the fish production. The use of antagonistic substances (bacteriocins) has been proven to be a viable option. The aim of this study was to evaluate different methods of purification for bacteriocin like inhibitory substances (BLIS). For the purification process, we isolated and used two Gram-positive bacilli that produce antagonistic substances for pathogens in aquaculture. Tests for detection of interfering factors were also performed. After the confirmation that the antagonistic action was due the BLIS activity, we carried out the purification methods. The methods tested were: cell free supernatant, acid extraction and ammonium sulfate precipitation at two concentrations (20 and 50%). Salmonella Tiphy CFP/IAL1472 and Aeromonas hydrophila (isolated in a tilapia production environment) were used as indicators of the efficiency of extracts in controlling pathogenic potentials. Ammonium sulfate precipitation at 50% was the most appropriate for purifying the antagonistic substance for both indicators. The extracts of the two isolates remained active for 22 days at 25ºC. These are promising results regarding the water and fish health without the use of antibiotics, in this manner being a safer environmental practice.(AU)
Técnicas para diminuir as perdas causadas por doenças bacterianas são importantes para melhorar continuamente a produção de pescado. O uso de substâncias antagônicas (bacteriocinas) tem-se mostrado uma opção viável. O objetivo do trabalho foi avaliar diferentes métodos de purificação de bacteriocinas como substâncias inibidoras (BLIS). Dois bacilos Gram-positivos, produtores de substâncias antagonistas para agentes patogênicos da aquicultura, foram utilizados em processos de purificação. Depois de confirmada a ação antagônica pela atividade de BLIS, os métodos de purificação foram realizados. Os métodos testados foram: células livres de sobrenadante, extração ácida e precipitação por sulfato de amônia em duas concentrações (20 e 50%). Salmonella Typhi PCP/IAL1472 e Aeromonas hydrophila (isolada de um ambiente de tilapicultura) foram utilizadas como indicadores de eficiência dos extratos. O precipitado por sulfato de amônio a 50% foi o mais adequado para purificar a substância antagonista para ambos os isolados indicadores. Os extratos dos dois isolados permaneceram ativos por 22 dias em 25ºC. Estes resultados são promissores do ponto de vista da manutenção da sanidade da água e dos peixes, sem uso de antibióticos, constituindo uma prática ambientalmente mais segura.(AU)
Assuntos
Pesqueiros/análise , Bacteriocinas/isolamento & purificação , Bacilos Gram-Positivos/isolamento & purificação , AquiculturaResumo
Specific proteases capable of degrading native triple helical or denatured collagen have been required for many years and have a large spectrum of applications. There are few complete reports that fully uncover production, characterization and purification of fungi collagenases. In this review, authors searched through four scientific on line data bases using the following keywords (collagenolytic OR collagenase) AND (fungi OR fungus OR fungal) AND (production OR synthesis OR synthesize) AND (characterization). Scientific criteria were adopted in this review to classify found articles by score (from 0 to 10). After exclusion criteria, 21 articles were selected. None obtained the maximum of 10 points defined by the methodology, which indicates a deficiency in studies dealing simultaneously with production, characterization and purification of collagenase by fungi. Among microorganisms studied the non-pathogenic fungi Penicillium aurantiogriseum and Rhizoctonia solani stood out in volumetric and specific collagenase activity. The only article found that made sequencing of a true collagenase showed 100% homology with several metalloproteinases fungi. A clear gap in literature about collagenase production by fungi was verified, which prevents further development in the area and increases the need for further studies, particularly full characterization of fungal collagenases with high specificity to collagen.(AU)
Assuntos
Fungos/isolamento & purificação , Fungos/enzimologia , Colágeno/genéticaResumo
Chaetoglobosin A is an antibacterial compound produced by Chaetomium globosum, with potential application as a biopesticide and cancer treatment drug. The aim of this study was to evaluate the feasibility of utilizing cornstalks to produce chaetoglobosin A by C. globosum W7 in solid-batch fermentation and to determine an optimal method for purification of the products. The output of chaetoglobosin A from the cornstalks was 0.34 mg/g, and its content in the crude extract was 4.80%. Purification conditions were optimized to increase the content of chaetoglobosin A in the crude extract, including the extract solvent, temperature, and pH value. The optimum process conditions were found to be acetone as the extractant, under room temperature, and at a pH value of 13. Under these conditions, a production process of the antifungal chaetoglobosin A was established, and the content reached 19.17%. Through further verification, cornstalks could replace crops for the production of chaetoglobosin A using this new production process. Moreover, the purified products showed great inhibition against Rhizoctonia solani, with chaetoglobosin A confirmed as the main effective constituent (IC50 = 3.88 µg/mL). Collectively, these results demonstrate the feasibility of using cornstalks to synthesize chaetoglobosin A and that the production process established in this study was effective.(AU)
Assuntos
Chaetomium , Zea mays , Antifúngicos/análise , Uso de Resíduos Sólidos , AntibacterianosResumo
Lactic acid, which can be obtained through fermentation, is an interesting compound because it can be utilized in different fields, such as in the food, pharmaceutical and chemical industries as a bio-based molecule for bio-refinery. In addition, lactic acid has recently gained more interest due to the possibility of manufacturing poly(lactic acid), a green polymer that can replace petroleum-derived plastics and be applied in medicine for the regeneration of tissues and in sutures, repairs and implants. One of the great advantages of fermentation is the possibility of using agribusiness wastes to obtain optically pure lactic acid. The conventional batch process of fermentation has some disadvantages such as inhibition by the substrate or the final product. To avoid these problems, this study was focused on improving the production of lactic acid through different feeding strategies using whey, a residue of agribusiness. The downstream process is a significant bottleneck because cost-effective methods of producing high-purity lactic acid are lacking. Thus, the investigation of different methods for the purification of lactic acid was one of the aims of this work. The pH-stat strategy showed the maximum production of lactic acid of 143.7 g/L. Following purification of the lactic acid sample, recovery of reducing sugars and protein and color removal were 0.28%, 100% and 100%, respectively.(AU)
Assuntos
Lacticaseibacillus rhamnosus/química , Lacticaseibacillus rhamnosus/enzimologia , Ácido LácticoResumo
O transplante de células germinativas é uma abordagem interessante para a conservação e reconstituição de espécies de peixes ameaçadas de extinção. Para realizar essa biotecnia, são necessários procedimentos espécie-específicos aplicados às espécies nativas. Este estudo teve como objetivo estabelecer técnicas de isolamento e criopreservação de oogônias-tronco de Brycon amazonicus, seguido de transplante em larvas triploides e transplante de células germinativas primordiais de Brycon amazonicus em embriões triploides (3N) e híbridos triploides (H3N). Para tal, as gônadas de B. amazonicus foram digeridas enzimáticamente e as células germinativas tronco foram separadas por gradiente descontinuo de densidade, e posteriormente foram purificadas e criopreservadas. As oogônias-tronco recém purificadas e criopreservadas de Brycon amazonicus foram marcadas com PKH26 e transplantadas na região da cavidade intraperitoneal em larvas triploides com 22 dias após a eclosão. Os resultados demonstraram que dez dias após o transplante de oogônias-tronco, foi possível identificar a presença das células doadoras em ambos tratamentos, no entanto, nos dias seguintes não foi observado a presença destas células nas cristas genitais dos hospedeiros. O transplante de células germinativas primordiais (PGCs) foram realizados utilizando as células GFP positivas no estágio de segmentação de B. amazonicus, nos embriões receptores 3N e H3N na região marginal lateral da blastoderme. Após o transplante, as células doadoras foram visualizadas durante todo o desenvolvimento embrionário, inclusive na eclosão, no entanto, não apresentaram migração e colonização. Este é o primeiro relato sobre o transplante de células germinativas utilizando larvas e embriões como receptores em espécies neotropicais. No entanto, para o nosso estudo, outros parâmetros devem ser otimizados para geração de quimeras germinativas e assim, poderão ser futuramente empregados em outras espécies nativas que estão em perigo de extinção ou de importância na aquicultura.
Germ cell transplantation is an interesting approach for the conservation and reconstitution of endangered fish species. To develop such biotechnique, species-specific studies are necessary to establish in native species. This study aimed to establish techniques for isolation and cryopreservation oogonial stem cells of Brycon amazonicus, followed by transplantation into triploid larvae and transplantation of primordial germ cells of Brycon amazonicus into triploid (3N) and triploid hybrids (H3N) embryos. Firstly, the gonads of B. amazonicus were enzymatically digested and the stem germ cells were isolated by a discontinuous density gradient, and later purified and cryopreserved. The newly purified and cryopreserved oogonial stem cells of Brycon amazonicus were labeled with PKH26 and transplanted intraperitoneallyinto triploid larvae 22 days after hatching. The results showed that ten days after oogonial stem cells transplantation, it was possible to identify the presence of donor cells in both treatments, however, in the following days, the presence of these cells in the host genital ridges was not observed. Transplantation of primordial germ cells (PGCs) was performed using GFP positive cells at the segmentation stage of B. amazonicus, in 3N and H3N recipient embryos in the lateral marginal region of the blastoderm. After transplantation, donor cells were visualized throughout embryonic development, including hatching, however, they did not show migration and colonization. This is the first report on germ cell transplantation using larvae and embryos as recipients in neotropical species. However, for our study, other parameters must be optimized for the generation of germline chimera and thus, may be used in the future in other enfangered native species or of importance in aquaculture.
Resumo
Immobilized lectins are a powerful biotechnological tool for separation and isolation of glycoconjugates. In the present study, polyvinyl alcohol (PVA) and glutaraldehyde (GA) were used as a support for Concanavalin A (Con A) covalent immobilization and for entrapment of Parkia pendula seed gum (PpeG). Con A immobilization yielded approximately 30% and 0.6 M glucose solution was the minimum concentration able to elute fetuin from column. PVA-GA-PpeG column was efficiently recognized by pure P. pendula lectin (PpeL). These findings indicate that PVA-GA interpenetrated network showed to be an efficient support for lectin covalent immobilization and as affinity chromatography matrix after trapping of PpeG.(AU)
Lectinas imobilizadas são uma poderosa ferramenta biotecnológica para a separação e isolamento de glicoconjugados. No presente trabalho álcool polivinílico (PVA) e glutaraldeído (GA) foram utilizados como um suporte para a imobilização covalente da Concanavalina A (Con A) e para aprisionamento da goma de semente de Parkia pendula (PpeG). A eficiência da imobilização da Con A foi aproximadamente 30 % e a concentração mínima de glucose capaz de eluir a fetuína da coluna foi 0,6 M. Coluna de PVA - GA - PpeG foi eficientemente reconhecida pela lectina de P. pendula (PpeL) pura. Estes resultados indicam que a rede interpenetrada de PVA-GA mostrou-se um suporte eficiente para a imobilização covalente de lectina e como matriz de cromatografia de afinidade após aprisionamento de PpeG.(AU)
Assuntos
Glutaral/análogos & derivados , Glutaral/análise , Cromatografia , LectinasResumo
As esponjas pertencem ao filo Porífera e são organismos multicelulares constituídos de células embebidas em uma matriz gelatinosa e enrijecidas por um esqueleto de espículas de carbonato de cálcio ou sílica e colágeno. O interesse nesse filo é inerente aos trabalhos relatados que mostram amplo potencial biotecnológico de macromoléculas com propriedades interessantes, mostrando atividade contra doenças e alguns patógenos, e possivelmente capazes de desempenhar o papel de ferramenta biomédica, como as lectinas. Lectinas são proteínas capazes de se ligarem reversivelmente a carboidratos específicos, sem que causem alterações estruturais nos mesmos. Estas proteínas são capazes de atuar como moléculas de reconhecimento no interior das células, superfícies celulares e fluidos fisiológicos. Em esponjas marinhas, as lectinas podem desempenhar uma variedade de funções, incluindo interação celular, espiculogênese e defesa. O objetivo deste trabalho foi detectar a atividade hemaglutinante em extratos proteicos de esponjas marinhas e purificar e caracterizar lectinas presentes nas esponjas marinhas Callyspongia vaginalis e Aplysina fulva. Os extratos das 11 espécies testadas apresentaram atividade hemaglutinante e hemolítica contra eritrócitos humanos e de coelho. Denominada de CvP (Callyspongia vaginalis Protein), a lectina de C. vaginalis foi isolada a partir de combinações cromatográficas de troca iônica em matriz de DEAE-sephacel e DEAE-FF. Esta proteína é composta de três cadeias polipeptídicas ligadas à um cromóforo com absorção a 600 nm. CvP compartilha alta similaridade de sequência com H-3, lectina isolada de Haliclona caerulea. Entretanto, CvP não apresentou atividade hemaglutinante, sendo assim, ela foi considerada uma lectin-like. AFL (Aplysina fulva Lectin), isolada de A. fulva, foi purificada através de precipitação com sulfato de amônio seguida de cromatografia de afinidade em matriz de Sepharose 4B. A nova lectina é um dímero de 30 kDa, formado por duas subunidades iguais de 15 kDa ligadas por pontes dissulfeto. Sua atividade hemaglutinante foi estável em pH neutro-alcalino e em temperaturas abaixo de 60ºC. A atividade de AFL foi inibida pela glicoproteína mucina de estômago de porco. AFL mostrou potencial na redução dos biofilmes das cepas bacteriana de Staphylococcus aureus, Staphylococcus epidermidis e Escherichia coli, sendo capaz de desempenhar papel antibacteriano. Assim, duas novas proteínas foram isoladas e caracterizadas bioquimicamente e os resultados apresentados acima servirão como base deaplicação biotecnológica em modelos biológicos diversos.
The sponges belong to the phylum Porífera and are multicellular organisms made up of cells embedded in a gelatinous matrix and stiffened by a skeleton of spicules of calcium carbonate or silica and collagen. The interest in this phylum is inherent in the studies reported that show broad biotechnological potential of macromolecules with interesting properties, showing activity against diseases and some pathogens, and possibly capable of playing the role of a biomedical tool, such as lectins. Lectins are proteins capable of reversibly binding to specific carbohydrates, without causing structural changes in them. These proteins are able to act as recognition molecules inside cells, cell surfaces and physiological fluids. In marine sponges, lectins can perform a variety of functions, including cell interaction, spiculogenesis and defense. The aim of this work was to detect hemagglutinating activity in protein extracts from marine sponges and to purify and characterize lectins present in marine sponges Callyspongia vaginalis and Aplysina fulva. The extracts of the 11 species tested showed hemagglutinating and hemolytic activity against human and rabbit erythrocytes. Called CvP (Callyspongia vaginalis Protein), the C. vaginalis lectin was isolated from chromatographic combinations of ion exchange in DEAE-sephacel and DEAE-FF matrix. This protein is composed of three polypeptide chains linked to a chromophore with absorption at 600 nm. CvP shares high sequence similarity with H-3, lectin isolated from Haliclona caerulea. However, CvP did not show hemagglutinating activity, so it was considered a lectin-like activity. AFL (Aplysina fulva Lectin), isolated from A. fulva, was purified by precipitation with ammonium sulfate followed by affinity chromatography on Sepharose 4B matrix. The new lectin is a 30 kDa dimer, formed by two equal 15 kDa subunits linked by disulfide bridges. Its hemagglutinating activity was stable at neutral-alkaline pH and at temperatures below 60ºC. AFL activity was inhibited by pig stomach mucin glycoprotein. AFL showed potential in reducing the biofilms of the bacterial strains of Staphylococcus aureus, Staphylococcus epidermidis and Escherichia coli, being able to play an antibacterial role. Thus, two new proteins were isolated and biochemically characterized and the results presented above will serve as a basis for biotechnological application in different biological models.
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An extracellular β-agarase was purified from
Assuntos
Adaptação Fisiológica/fisiologia , Ágar/metabolismo , /metabolismo , Pseudoalteromonas/enzimologia , Adaptação Fisiológica/genética , Regiões Antárticas , Proteínas de Bactérias/metabolismo , Temperatura Baixa , Dissacarídeos/biossíntese , Sedimentos Geológicos/microbiologia , Glicosídeo Hidrolases/isolamento & purificação , Hidrólise , /genéticaResumo
Abstract Lipases are enzymes of immense industrial relevance, and, therefore, are being intensely investigated. In an attempt to characterize lipases at molecular level from novel sources, a lipase gene from Bacillus amyloliquefaciens PS35 was cloned, heterologously expressed in Escherichia coli DH5α cells and sequenced. It showed up to 98% homology with other lipase sequences in the NCBI database. The recombinant enzyme was then purified from E. coli culture, resulting in a 19.41-fold purification with 9.7% yield. It displayed a preference for long-chain para-nitrophenyl esters, a characteristic that is typical of true lipases. Its optimum pH and temperature were determined to be 8.0 and 40 °C, respectively. The half-lives were 2.0, 1.0 and 0.5 h at 50 °C, 60 °C and 70 °C, respectively. The metal ions K+ and Fe3+ enhanced the enzyme activity. The enzyme displayed substantial residual activity in the presence of various tested chemical modifiers, and interestingly, the organic solvents, such as n-hexane and toluene, also favored the enzyme activity. Thus, this study involves characterization of B. amyloliquefaciens lipase at molecular level. The key outcomes are novelty of the bacterial source and purification of the enzyme with desirable properties for industrial applications.(AU)
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Bacillus/classificação , Bacillus/crescimento & desenvolvimento , Lipase , Proteínas Recombinantes/biossíntese , Proteínas Recombinantes/metabolismoResumo
Venom hyaluronidase (Hyase) contributes to the diffusion of venom from the inoculation site. In this work, we purified and characterized Hyase from the venom of Vitalius dubius (Araneae, Theraphosidae), a large theraphosid found in southeastern Brazil. Venom obtained by electrical stimulation of adult male and female V. dubius was initially fractionated by gel filtration on a Superdex® 75 column. Active fractions were pooled and applied to a heparin-sepharose affinity column. The proteins were eluted with a linear NaCl gradient.(AU)
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Animais , Hialuronoglucosaminidase/análise , Venenos/administração & dosagem , Aranhas/classificaçãoResumo
Laccases are blue copper oxidases (E.C. 1.10.3.2) that catalyze the one-electron oxidation of phenolics, aromatic amines, and other electron-rich substrates with the concomitant reduction of O2 to H2O. A novel laccase gene pclac2 and its corresponding full-length cDNA were cloned and characterized from Phytophthora capsici for the first time. The 1683 bp full-length cDNA of pclac2 encoded a mature laccase protein containing 560 amino acids preceded by a signal peptide of 23 amino acids. The deduced protein sequence of PCLAC2 showed high similarity with other known fungal laccases and contained four copper-binding conserved domains of typical laccase protein. In order to achieve a high level secretion and full activity expression of PCLAC2, expression vector pPIC9K with the Pichia pastoris expression system was used. The recombinant PCLAC2 protein was purified and showed on SDS-PAGE as a single band with an apparent molecular weight ca. 68 kDa. The high activity of purified PCLAC2, 84 U/mL, at the seventh day induced with methanol, was observed with 2,2'-azino-di-(3-ethylbenzothialozin-6-sulfonic acid) (ABTS) as substrate. The optimum pH and temperature for ABTS were 4.0 and 30 ºC, respectively . The reported data add a new piece to the knowledge about P. Capsici laccase multigene family and shed light on potential function about biotechnological and industrial applications of the individual laccase isoforms in oomycetes.(AU)
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Lacase/genética , Lacase/metabolismo , Phytophthora/enzimologia , Clonagem Molecular , Sequência Conservada , Estabilidade Enzimática , Expressão Gênica , Concentração de Íons de Hidrogênio , Lacase/química , Lacase/isolamento & purificação , Peso Molecular , Fases de Leitura Aberta , Estrutura Terciária de Proteína , Phytophthora/genética , Pichia/genética , Sinais Direcionadores de Proteínas/genética , Proteínas Recombinantes/química , Proteínas Recombinantes/genética , Proteínas Recombinantes/isolamento & purificação , Proteínas Recombinantes/metabolismo , Homologia de Sequência de Aminoácidos , TemperaturaResumo
In the present study, a bacterium isolated from Marcha- a herbal cake used as traditional starter culture to ferment local wine in North East India, was evaluated for bacteriocin like inhibitory substance production and was tested against six food borne/spoilage causing pathogens viz. Listeria monocytogenes MTCC 839, Bacillus subtilis MTCC 121, Clostridium perfringens MTCC 450, Staphylococcus aureus, Lactobacillus plantarum and Leuconostoc mesenteroides MTCC 107 by using bit/disc method followed by well diffusion method. The bacterial isolate was identified as Brevibacillus borstelensis on the basis of phenotypic, biochemical and molecular characteristics using 16Sr RNA gene technique. Bacteriocin like inhibitory substance produced by Brevibacillus borstelensis AG1 was purified by gel exclusion chromatography. The molecular mass of the Brevibacillus borstelensis AG1 was found to be 12 kDa. Purified bacteriocin like inhibitory substance of Brevibacillus borstelensis was further characterized by studying the effect of temperature, pH, proteolytic enzyme and stability. Bacteriocin like inhibitory substance was found to be thermostable upto 100 °C, active at neutral pH, sensitive to trypsin, and partially stable till third week of storage thus showing a bright prospective to be used as a potential food biopreservative.