Single-Copy Insertion of Split-GFP for the Restriction of Germline Expression in Caenorhabditis elegans

Al Johani, Mohammed

11 1900

Gene regulation in C. elegans germ cells depend on transgenerational chromatin modification and small RNA pathways. Germline silencing mechanisms evolved to repress foreign DNA from compromising the transfer of genetic information to progeny. Effective genetic tools that circumvent the silencing machinery will facilitate studies using this model organism. Specifically, translation of heat-shock inducible transgenes is inhibited in the germline making it challenging to transiently express enzymes to modify the genome. Here, we describe a genetic screen design that can be used to identify pathways that prevent germline expression of heat-shock induced transgenes. We use split-GFP (GFP1-10 and GFP11) to confine a genetic screen to germ cells. Stable transgenic lines with germline expression of single-copy integrated GFP11 were produced using MosSCI. The insertion lines will be used in RNAi or chemical mutagenesis screens for the germline de-repression of GFP1-10 expressed under heat-shock promoters. The screen is likely to identify candidate RNAi or chromatin factors involved in repressing heat-shock expression in the germline, particularly from extrachromosomal arrays. Inducible high-level expression in the germline from extrachromosomal arrays would be a valuable tool for large-scale genome engineering.

Caenorhabditis elegans

Germline

Split-GFP

Synthetic Biology

Monitoring the Expression of rrn Operons by Novel Gfp Reporter System in Model Drinking Water

Chen, Yanping

27 September 2005

No description available.

Engineering, Environmental

rrn operon

Gfp

Rfp

Farnesyltransferase: Gene Expression in Plants and Role in Plant Development

Zhou, Dafeng

14 March 1997

Protein farnesyltransferase (FTase, E. C. 2.5.1.21) post-translationally modifies regulatory proteins involved in controlling cell growth, division, and differentiation. Recently, a cDNA clone (PsFTb) encoding a pea (Pisum sativum) FTase b subunit was isolated. Initial studies led to the hypothesis that FTase plays a role in the regulation of plant cell division. To gain insight into FTase function in plants, a detailed study of the expression pattern of FTase genes was carried out. A cDNA (NgFTb) encoding the b subunit of tobacco FTase was cloned from a Nicotiana glutinosa cDNA library to initiate studies in tobacco. In tobacco BY-2 suspension culture, levels of NgFTb mRNA and FTase activity transiently increased at the early log phase of cell growth and rapidly declined before cells entered stationary phase. These data, along with inhibitor studies in the BY-2 system, support our hypothesis. To understand the expression and regulation of pea FTase subunit genes, 5'-upstream sequences of both pea FTase subunit genes (PsFTb and PsFTa) were cloned from a pea genomic library. The 5'-upstream sequence (~2 kb) of PsFTa was fused to GUS (b-glucuronidase) and GFP (green fluorescent protein) reporter genes and introduced into tobacco plants. This 2 kb upstream region appears insufficient to provide PsFTa promoter function. On the other hand, 3.2 kb of PsFTb 5'-upstream sequence expressed as a PsFTb:GUS construct is fully functional in transgenic tobacco plants. GUS expression was most prominent in actively growing cells supporting FTase involvement in plant cell cycle control. GUS activity was also found in mature and imbibed embryos but not premature embryos, consistent with the role of FTase in abscisic acid (ABA) signaling. An unexpected pattern of GUS activity, not correlated with dividing cells or ABA signaling, was also observed in the transgenic plants. GUS activity was detected in vascular bundles adjacent to actively-growing tissues and in regions that connect two organs, e.g., junctions between stems and leaf petioles, cotyledons and hypocotyls, roots and hypocotyls. Auxin promotes PsFTb expression while light and sucrose inhibit expression. These spatial and temporal expression patterns strongly suggest that FTase has a broader role associated with regulation of nutrient transportation or allocation in plants. / Ph. D.

Farnesyltransfe

Expression

GUS

Prenylation

GFP

Isoprenoid

cDNA?GFP Fusion Libraries for Analyses of Protein Localization in Mouse Stem Cells

Murray, Heather

January 2005

Stem cells have great potential value for treating a number of diseases and conditions, including diabetes, Parkinson's, and spinal cord injuries. Applying stem cells for therapeutic purposes will require an in-depth understanding of their biology, not only of the genes they express, but also the functions of the proteins encoded by the genes. The goal of the project presented in this thesis was to develop a method for high-throughput analyses of protein localization in mouse stem cells. Localization information can provide insight into the functions and biological roles of proteins. <br /><br /> One means of studying protein localization involves creating proteins with a green fluorescent protein (GFP) reporter gene and analyzing their localization using fluorescence microscopy. The research outlined in this thesis focused on developing a system to create a large number of GFP-tagged proteins by constructing a cDNA?GFP fusion library. This involved exploring methods for optimizing cDNA synthesis, designing a retroviral vector (pBES23) for the expression of cDNA?GFP fusions in mouse stem cells, and constructing a cDNA?GFP fusion library in this vector using R1 mouse embryonic stem cell mRNA. The library constructed was not successfully delivered to target cells for GFP-tagged protein expression; it was therefore not possible to characterize protein localization in mouse stem cells. Suggestions are given as to how the methods used in this thesis might be optimized further.

Biology

protein localization

green fluorescent protein

GFP

stem cells

cDNA-GFP fusion library

Transfert du CFTR par vecteurs de gènes dérivés des adénovirus ou par trogocytose de microparticules membranaires : mécanismes moléculaires et applications à la mucoviscidose / Transfer of CFTR by gene tranfer vectors derived from adenoviruses or by trogocytosis of membrane-derived microparticle : molecular mechanisms and applications in cystic fibrosis

Gonzalez, Gaëlle

14 December 2011

La mucoviscidose est une maladie génétique due à des mutations du gène CFTR, conduisant à une altération de la fonction de canal à ions chlorure de la glycoprotéine transmembranaire CFTR associée à une atteinte pulmonaire sévère. Plusieurs études récentes ont amené à reconsidérer l’utilisation des vecteurs adénoviraux (Ad) de sérotype 5 (Ad5) dans la mucoviscidose, lesquels induisent non seulement des réactions immunes anti-adénovirales mais aussi des effets cytopathiques indésirables. (1) Dans une première partie de notre étude, nous avons étudié l’entrée et le transit intracellulaire de l’Ad5/F35, vecteur chimérique portant les fibres de l’Ad sérotype 35 sur une capside de sérotype 5. Nous avons montré que la protéine fibre est déterminante dans l’internalisation et le trafic intracellulaire de ce vecteur. Le vecteur Ad5/F35 exprimant la fusion GFP-CFTR s’est révélé (i) être dépourvu de cytotoxicité, (ii) transduire efficacement les cellules épithéliales pulmonaires par voie apicale, et (iii) restaurer l’activité de canal à chlorure dans les cellules CFTR(-). Il constitue donc un vecteur de transfert du gène CFTR potentiellement utilisable en thérapie génique de la mucoviscidose. (2) Dans une seconde partie, nous avons exploré une stratégie alternative de transfert de la protéine CFTR par trogocytose. Nous avons fait l’hypothèse que le canal CFTR pouvait être véhiculé par des microvésicules ou microparticules membranaires (MP) émanant de la membrane cellulaire et libérées dans le milieu de culture. En utilisant un système d’expression stable de la protéine CFTR étiquetée par la protéine fluorescente GFP (GFP-CFTR) dans des cellules donneuses, nous avons pu démontrer que les MP sont capables de prendre en charge et délivrer la protéine GFP-CFTR à des cellules réceptrices, mais ce transfert n’est assuré que par une population réduite de MP (≤ 8 %), et la durée de vie du GFP-CFTR n’est que transitoire (≤ 24h). En fait, la majorité des MP transfèrent des molécules d’ARN messager ou polysomal GFP-CFTR. La protéine GFP-CFTR néosynthétisée à partir de ces ARNm est exprimée plus tardivement (> 48h) mais de façon prolongée (≥ 10 jours). La fonctionnalité du canal CFTR ainsi néosynthétisé est en cours d’évaluation. Les MP constituent donc un nouveau type de vecteurs de transfert non génique du CFTR qui pourraient être employés en thérapie de la mucoviscidose. / The cystic fibrosis (CF) is a genetic disease due to mutations of the CFTR gene, resulting in the alteration of the Cl channel function carried by the transmembranal glycoprotein CFTR, and associated with severe pulmonary complications. Several recent studies led the medical and scientific community to reconsider the use of adenovirus serotype 5 (Ad5)-based vectors as CFTR gene transfer vectors in CF gene therapy. Not only immune response against the vector itself and the ansduced cells have been observed, but also Ad5-induced nondesired cytopathic effects. (1) In the first part of our study, we analyzed the cell entry and traficking of Ad5/F35, a chimeric vector consisting of serotype 5 capsid carrying serotype 35 fibers. We showed that the fibre protein is the major, if not only, determinant of the internalisation and entry pathway of Ad5/F35. Ad5/F35-GFP-CFTR, expressing the fusin protein GF-CFTR, was found (i) to be devoid of detectable cytopathic effect, (ii) efficiently transduced airway epithélial cells via the apical pole, and (iii) restore the Cl channel function in CF cells. Ad5/F35 therefore represents a CFTR gene transfer vector with a great potential for gene therapy of CF. (2) In the second part of our study, we have investigated an alternative strategy based on the transfer of the mature CFTR protein via trogocytosis. We hypothesized that microvesicles or microparticules (MP) issued from the cell membranes and released into the culture medium could transport and achieve the cell-to-cell transfer of CFTR channel cargo. We engineered donor cells for stable expression of GFP-tagged CFTR protein (GFP-CFTR), and showed that donor cell-issued MP were capable of delivering GFP-CFTR protein to recipient cell. However, the GFP-CFTR protein was only transferred by a limited population of MP (≤ 8 %), and was only transient (≤ 24h). In fact, the major population of MP transferred mRNAGFP-CFTR or polysomal thereof. Interestingly, the GFPCFTR protein newly synthesized from this mRNAGFP-CFTR was expressed at late times after transfer (≥ 48 h) but in a prolonged manner (≥ 10 jours). The Cl canal function after MP-mediated CFTR transfer is being evaluated. MP represent a novel type of CFTR vectors which can be produced by specifically designed autologous donor cells, and which would overcome most of the inconveniences of gene therapy using viral or nonviral vectors.

Adénovirus

Microparticule membranaire

GFP-CFTR

Trogocytose

Exosome

Adenovirus

Microparticle membrane

GFP-CFTR

Trogocytosis

Exosome

616.9101

Estudo comparativo de promotores de micobactérias utilizando GFP como gene repórter para o desenvolvimento de vacinas de BCG recombinante. / Comparative study of mycobacterial promoters using GFP as a reporter gene for the development of recombinant BCG vaccines.

Nascimento, Larissa Vilela

07 August 2015

BCG é uma das vacinas mais usadas no mundo. Avanços na manipulação genética têm permitido o seu uso como carreador de antígenos heterólogos, porém o aprimoramento dos sistemas de expressão se faz necessário, sendo o promotor um importante elemento, uma vez que regula o nível de produção do antígeno, induzindo uma resposta imunológica adequada. Avaliamos a atividade de diferentes promotores de micobactérias, como o PAg, PAN, PBlaF*, Phsp60 e um promotor ainda não caracterizado do micobacteriófago L5, usando o gene gfp como repórter da expressão, todos clonados no vetor extracromossomal, pLA71. Foi possível avaliar as cepas de M. smegmatis e BCG fluorescentes para quase todas as construções e alguns plasmídeos pLA71-p mostraram características diferentes dependentes da micobactéria transformada. Numa escala de força de expressão, os diferentes promotores se apresentaram como fraco (pLA71-PAN-gfp), médio (pLA71-PBlaf*-gfp) e forte (pLA71-Phsp60-gfp). Os rBCG foram usados para infecção de macrófagos e a atividade dos promotores não foi afetada após a internalização. Para ensaio de localização, camundongos foram inoculados com BCG e foi possível confirmar a presença de colônias (recombinantes ou não) nos pulmões após 1 e 3 dias de inoculação, por plaqueamento em meio sólido e por microscopia confocal. / BCG is one of the most widely used vaccines in the world. Advances in genetic manipulation have allowed their use as a carrier for heterologous antigens, however the improvement of systems of expression is necessary, the promoter being an important element, since it regulates the expression level of the antigen, inducing an adequate immune response. We evaluated the activity of different promoters of mycobacteria, such as PAg, PAN, PBlaF* and Phsp60, and the not yet characterized promoter of the micobacteriophage L5, using GFP as a reporter gene expression activity, all cloned in the extrachromosomal vector, pLA71. It was possible to evaluate promoters in the M. smegmatis and BCG strains, fluorescent for almost all constructions and some pLA71-p plasmids showed different characteristics dependent on the transformed mycobacterium. The different promoters showed expression levels as weak (pLA71-PAN-gfp), medium (pLA71-PBlaf*-gfp) and strong (pLA71-Phsp60-gfp). The rBCG were used for infection of macrophages and the activity of the promoters wasnt affected after internalization. For BCG location test, mice were inoculated and it was possible to confirm the presence of colonies (recombinant or not) in the lungs after 1 and 3 days after inoculation by plating on solid medium and by confocal microscopy.

Green fluorescent protein (gfp)

Micobactérias

Mycobacteria

Promoters of expression

Promotores de expressão

Proteína verde fluorescente (gfp)

Interação entre proteínas fluorescentes e nanocristais de CdSe/ZnS / Interaction between fluorescent proteins and CdSe/ZnS nanocrystals

Hering, Vitor Renaux

01 June 2007

Foram utilizadas proteínas da famÌlia das GFPs e nanocristais fluorescentes de CdSe/ZnS para caracterização da interação e verificação de transferência de energia por ressonância (FRET) entre estes compostos. Formou-se dois pares doador-receptor onde ora uma proteína figurava como doadora, ora um nanocristal ocupava este papel. Verificou-se que, em ambos os casos, o doador sofre supressão da fluorescência após a formação de complexo com o receptor, complexo este motivado por interação eletrostática e dependente de pH. Foi possível comprovar, através da observação de emissão sensitizada e redução da anisotropia, que entre o par formado por nanocristal com emissão no verde e proteína HcRed1 como receptora, de fato ocorre FRET. As distâncias aparentes entre doador e receptor foram determinadas a partir da eficiência da supressão da fluorescência do doador e da distância de Förster. As distâncias assim obtidas são compatíveis com as dimensões das proteínas e dos nanocristais / Proteins belonging to the GFP family were used to characterize their interaction with fluorescent CdSe/ZnS nanocrystals and to verify the occurrence of resonance energy transfer (FRET) among these elements. Two donor-acceptor pairs were established, one having a protein as donor and the other having a nanocrystal as donor. In both cases the donor suffers quenching of its fluorescence after the formation of a complex with the acceptor. The complex formation is dependent on pH and is due to electrostatic interaction. It was possible to prove the occurrence of FRET between CdSe/ZnS nanocrystals emitting green fluorescence as donors and the protein HcRed1 as acceptor, through the detection of sensitized emission and anisotropy reduction. Apparent donor-acceptor distances were determined from efficiency measurements and Förster distances. The obtained distances agreed with the protein and nanocrystal dimensions

CdSe/ZnS

CdSe/ZnS

Fluorescent proteins

FRET

FRET

GFP

GFP

HcRed1

HcRed1

Nanocristais

Nanocrystals

ProteÌnas fluorescentes

Estudos de renaturação de proteínas agregadas utilizando altas pressões hidrostáticas / Renaturation studies of aggregate proteins using high hydrostatic pressure

Natália Malavasi Vallejo

05 March 2013

No presente trabalho estudamos a renaturação sob alta pressão hidrostática de uma forma mutante da proteína verde fluorescente (enhanced GFP, eGFP), a qual somente emite fluorescência característica quando enovelada na sua forma nativa. A abordagem do presente estudo foi focada no controle da bioatividade da proteína recombinante, a fluorescência, como alternativa à determinação de solubilidade da proteína, fator que não é um indicador ideal de enovelamento proteico adequado. A ação da alta pressão na solubilização dos corpos de inclusão (CI) de eGFP produzidos em bactérias E. coli recombinantes e no enovelamento da proteína foi estudada. A compressão dos CI de eGFP em 2,4 kbar durante 30 minutos promoveu a dissociação dos agregados. No entanto, a incubação nesta condição não favoreceu o enovelamento da eGFP. O processo de renaturação foi avaliado em diversas condições de descompressão após a dissociação em 2,4 kbar. Durante a descompressão gradual, o aumento da fluorescência foi obtido em pressões que variaram entre a pressão atmosférica e 1,38kbar. Os níveis mais elevados de fluorescência de eGFP foram obtidos por incubação durante várias horas a níveis de pressão entre 0,35 e 0,69 kbar. Esta condição de pressão se mostrou favorável à renaturação de eGFP e é possível que também possa ser utilizada para favorecer o enovelamento de outras proteínas monoméricas. Ainda utilizando a eGFP como modelo, verificamos que os CI desta proteína produzidos por bactérias cultivadas em menor temperatura (37ºC) possuem maior quantidade de proteína recombinante apresentando a fluorescência característica em 509 nm, ou seja, na sua forma nativa, do que os CI expressos em temperaturas mais elevadas (42ºC e 47ºC). A análise realizada por espectroscopia de infravermelho (FT-IR) também demonstrou que os CI produzidos em temperaturas mais brandas possuem maior grau de estruturas secundárias semelhantes às da proteína na sua forma nativa. Além disso, os CI produzidos a 37ºC também são mais facilmente solubilizados pela ação da alta pressão do que aqueles produzidos em maior temperatura. Conforme esperado, a renaturação da eGFP a partir de CI produzidos a 37ºC foi 25 vezes mais eficiente do que a obtida utilizando CI produzidos a 47ºC. No presente estudo demonstramos também que a dissociação dos agregados exercida pela ação da alta pressão (2,4 kbar) pode ser amplificada quando em associação com a incubação em baixa temperatura (-9ºC) e que a combinação destas duas propriedades físicas eleva a solubilização dos agregados em CI, com a consequente elevação dos rendimentos de renaturação de eGFP. Mostramos ainda no presente estudo que a cinética de renaturação de eGFP em 0,69 kbar é proporcional à temperatura de incubação (entre 10ºC e 50ºC). O nível mais elevado de fluorescência foi obtido quando a renaturação de eEGP foi realizada a 20ºC. A taxa de maturação do cromóforo da eGFP é mais fortemente afetada pela temperatura do que a taxa de enovelamento da proteína. Em conclusão, a temperatura de produção dos CI, a temperatura de dissociação dos agregados e a temperatura de enovelamento podem afetar muito o rendimento e a cinética da renaturação de eGFP em alta pressão. Os resultados do presente estudo podem abrir novas perspectivas para melhorias no processo de enovelamento de proteínas a partir de CI utilizando alta pressão. Também neste trabalho descrevemos a renaturação das proteínas de Xac, PilB e os produtos dos genes XAC2810 e XAC3272 nunca antes obtidas na forma solúvel. Os rendimentos de solubilização destas três proteínas foram muito altos, entre 75% e 89%. A proteína PilB renaturada em alta pressão apresentou atividade ATPasica elevada, o que nunca antes foi demonstrado para a PilB de Xac. / In the present work we studied the refolding under high hydrostatic pressure of a mutant form of the green fluorescent protein (eGFP), which only emits the green characteristic fluorescence when in the native folded state. The approach of the present study was focused on controlling the bioactivity of the recombinant protein, the fluorescence, as an alternative for the determination of protein solubility, which is not an ideal indicator of proper protein folding. We studied the action of high pressure in the solubilization of the inclusion bodies (IB) of eGFP produced in bacteria E. coli and in the folding of this protein. The compression of a suspension of eGFP IB at 2.4 kbar for 30 minutes promoted dissociation of aggregates. However, the eGFP folding, monitored by the fluorescence at 509 nm, does not occur in this pressure level. The process of eGFP refolding was evaluated under various decompression conditions after dissociation of the IB at 2.4 kbar. During the gradual decompression, the increase in fluorescence was achieved at pressures ranging between atmospheric pressure and 1.38 kbar. The higher levels of eGFP fluorescence were obtained by incubation for several hours at pressure levels between 0.35 and 0.69 kbar. It is possible that the pressure condition that proved favorable for refolding of eGFP can also be used to favor the folding of other monomeric proteins. Using eGFP as a model, we also found that the IB produced by bacteria grown in a relatively low temperature (37ºC) is more fluorescent, presenting a higher amount of recombinant protein with the characteristic fluorescence at 509 nm, i.e., in its native form, than the IB expressed at higher temperatures (42ºC and 47ºC). The analysis by infrared spectroscopy (FT-IR) also demonstrated that the IB produced at milder temperatures have a higher degree of secondary structure similar to the protein in its native form. Furthermore, the IB produced at 37ºC are also more readily solubilized by the action of high pressure than those produced at the higher temperatures. As expected, the folding of eGFP from IB produced at 37ºC was 25 times more efficient than that obtained using IB produced at 47ºC. In this study we demonstrated that the dissociation of aggregates exerted by the action of high pressure (2.4 kbar) can be amplified by combination with incubation at low temperature (-9ºC) and the association of these two physical properties can be used to increase the solubilization of the aggregates in IB, with a consequent increase in the yield of eGFP refolding. In the present study we also showed that the kinetics of refolding of eGFP is proportional to temperature (10ºC 50ºC). The higher level of fluorescence was obtained when the refolding of eGFP was performed at 20°C. The rate of maturation of the eGFP chromophore is more strongly affected by temperature than the rate of folding of the protein. In conclusion, the temperature of production of IB, the temperature of dissociation of aggregates and the folding temperature can greatly affect the yield and kinetics of refolding of eGFP at high pressure. The results of this study may open new perspectives for improvements in the process of protein folding from IB using high pressure. In this paper we also describe the refolding of the proteins of Xac, PilB and the gene products XAC2810 and XAC3272, which have never before been achieved in soluble form. The yields of solubilization/refolding of these three proteins were very high, between 75% and 89%. The protein PilB refolded at high pressure presented high ATPase activity, which has never been shown for the PilB of Xac.

altas pressões hidrostáticas

corpos de inclusão

GFP

proteínas

renaturação

GFP

high hydrostatic pressure

inclusion bodies

proteins

refolding

Construção de sistema de aquecimento ôhmico e verificação comparativa do comportamento da proteína verde fluorescente e da bacteriocina nisina quando sob aquecimento convencional e ôhmico / Construction of an ohmic heating equipment and comparative analysis of green fluorescent protein fluorescence decay and nisin activity loss under conventional and ohmic heating

Marcos Camargo Knirsch

04 February 2011

Os processos de tratamento térmico por meio do aquecimento ôhmico revelam-se bastante promissores. A tecnologia de processamento de alimentos através do aquecimento ôhmico tem mostrado a obtenção de um produto final com características sensoriais e nutricionais superiores, quando comparada aos métodos convencionais (trocadores de calor ou banho de água). A principal vantagem atribuída ao aquecimento ôhmico é a habilidade de aquecer materiais rapidamente e de modo uniforme possibilitando desta forma a redução do abuso térmico aos produtos. A construção de um equipamento de aquecimento ôhmico foi realizada e seu funcionamento avaliado. Alguns pontos críticos para o funcionamento do equipamento foram encontrados e avaliados. Dentre os principais pontos críticos avaliados estão: o sistema de medição de temperatura e a distribuição dos campos elétricos. A avaliação destes pontos críticos possibilitou a realização de novo projeto de equipamento com o objetivo de otimizar a aplicação do aquecimento ôhmico. Realizou-se estudo comparativo da velocidade de inativação da fluorescência da proteína verde fluorescente (GFPuv) e da inativação da atividade da bacteriosina nisina, quando submetidas a aquecimento convencional (banho d\'água) e ôhmico, com o objetivo de avaliar a influencia da presença de campos elétricos. Leituras em &#955;ex = 394 nm, &#955;em = 509 nm para excitação e emissão respectivamente para a GFPuv e avaliação por halo de inibição para a atividade da nisina foram realizadas periodicamente após tratamento térmico por metodologia convencional e ôhmica a temperaturas de 60º, 70º e 80ºC para GFPuv e de 70ºe 80ºC para a nisina. Os resultados indicam que para ambos, GFP e nisina, a presença de campos elétricos não influencia de modo significativo o comportamento quando comparada a tecnologia de aquecimento ôhmico e convencional. / Ohmic heating is an emerging technology that possesses many actual and future applications. One of the most promising applications for this technology is food processing. Ohmic heating has demonstrated to achieve better sensorial and nutritional values when compared to conventional heating (heat exchangers/water bath). The principal advantage of ohmic heating is the ability to heat materials rapidly and uniformly making possible to reduce thermal abuse to products. An ohmic heating equipment was constructed and evaluated. Critical functioning points were observed on the manufactured equipment and were evaluated. Among the observed critical points include the temperature measurement system and the distribution of the electric fields on the extension of the equipment\'s container. As a result of the evaluation of those critical points a new equipment project was created aiming to optimize the ohmic heating unit. The influence of the electric field over the fluorescence decay of the green fluorescent protein (GFPuv) and over nisin activity decay was evaluated. Fluorescence readings were performed at &#955;ex = 394 nm, &#955;em = 509 nm for excitation and emission respectively for GFPuv and activity readings were performed by inhibition halo for nisin after several thermal treatment periods on ohmic and conventional heating. Samples were heated by conventional and ohmic heating at 60º, 70º and 80ºC for GFPuv and at 70º, 80º and 90ºC for nisin. The observed results indicate that the incidence of electric fields did not presented significative influence on the fluorescence decay of GFPuv or on the activity of nisin when ohmic heating was compared with conventional heating.

Aquecimento ôhmico

GFP

Nisina

Processamento de alimentos

Food processing

GFP

Nisin

Ohmic heating

Construção de sistema de aquecimento ôhmico e verificação comparativa do comportamento da proteína verde fluorescente e da bacteriocina nisina quando sob aquecimento convencional e ôhmico / Construction of an ohmic heating equipment and comparative analysis of green fluorescent protein fluorescence decay and nisin activity loss under conventional and ohmic heating

Knirsch, Marcos Camargo

04 February 2011

Os processos de tratamento térmico por meio do aquecimento ôhmico revelam-se bastante promissores. A tecnologia de processamento de alimentos através do aquecimento ôhmico tem mostrado a obtenção de um produto final com características sensoriais e nutricionais superiores, quando comparada aos métodos convencionais (trocadores de calor ou banho de água). A principal vantagem atribuída ao aquecimento ôhmico é a habilidade de aquecer materiais rapidamente e de modo uniforme possibilitando desta forma a redução do abuso térmico aos produtos. A construção de um equipamento de aquecimento ôhmico foi realizada e seu funcionamento avaliado. Alguns pontos críticos para o funcionamento do equipamento foram encontrados e avaliados. Dentre os principais pontos críticos avaliados estão: o sistema de medição de temperatura e a distribuição dos campos elétricos. A avaliação destes pontos críticos possibilitou a realização de novo projeto de equipamento com o objetivo de otimizar a aplicação do aquecimento ôhmico. Realizou-se estudo comparativo da velocidade de inativação da fluorescência da proteína verde fluorescente (GFPuv) e da inativação da atividade da bacteriosina nisina, quando submetidas a aquecimento convencional (banho d\'água) e ôhmico, com o objetivo de avaliar a influencia da presença de campos elétricos. Leituras em &#955;ex = 394 nm, &#955;em = 509 nm para excitação e emissão respectivamente para a GFPuv e avaliação por halo de inibição para a atividade da nisina foram realizadas periodicamente após tratamento térmico por metodologia convencional e ôhmica a temperaturas de 60º, 70º e 80ºC para GFPuv e de 70ºe 80ºC para a nisina. Os resultados indicam que para ambos, GFP e nisina, a presença de campos elétricos não influencia de modo significativo o comportamento quando comparada a tecnologia de aquecimento ôhmico e convencional. / Ohmic heating is an emerging technology that possesses many actual and future applications. One of the most promising applications for this technology is food processing. Ohmic heating has demonstrated to achieve better sensorial and nutritional values when compared to conventional heating (heat exchangers/water bath). The principal advantage of ohmic heating is the ability to heat materials rapidly and uniformly making possible to reduce thermal abuse to products. An ohmic heating equipment was constructed and evaluated. Critical functioning points were observed on the manufactured equipment and were evaluated. Among the observed critical points include the temperature measurement system and the distribution of the electric fields on the extension of the equipment\'s container. As a result of the evaluation of those critical points a new equipment project was created aiming to optimize the ohmic heating unit. The influence of the electric field over the fluorescence decay of the green fluorescent protein (GFPuv) and over nisin activity decay was evaluated. Fluorescence readings were performed at &#955;ex = 394 nm, &#955;em = 509 nm for excitation and emission respectively for GFPuv and activity readings were performed by inhibition halo for nisin after several thermal treatment periods on ohmic and conventional heating. Samples were heated by conventional and ohmic heating at 60º, 70º and 80ºC for GFPuv and at 70º, 80º and 90ºC for nisin. The observed results indicate that the incidence of electric fields did not presented significative influence on the fluorescence decay of GFPuv or on the activity of nisin when ohmic heating was compared with conventional heating.

Aquecimento ôhmico

Food processing

GFP

GFP

Nisin

Nisina

Ohmic heating

Processamento de alimentos