930 resultados para silver-stained denaturing PAGE
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Inside this Issue: Spring Service LearningWhy I Teach HonorsHonors Course ReflectionsHonors LifeWays to Get InvolvedHonors Study Abroad SpotlightBigs and Littles
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Inside this Issue: Why I Teach HonorsHonors SymposiaSpring 2013 HonorsA Semester in PicturesFall Service LearningWhy I Chose HonorsWhat Honors Continues to Do For MeHonorable MentionsAcademia Achieved: A Reflection on Fall 2012Student Spotlight: Matthew NealHonors with International Experience: IndiaCongratulations December 2012 Graduates!
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Inside this Issue: Fall Service LearningWhy I Teach HonorsCongratulations May 2012 Graduates!WUHA! - A Semester in PicturesNew WUHA! OfficersHonors Educational Experiences Student Spotlight: Austin Bischoff 6 Study Abroad
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Inside this Issue: Student Spotlight: David ThackhamSpring 2012 CoursesCongratulations December 2011 Graduate!ConnectED Nicaragua WUHA! - A Semester in PicturesReflection on Fall 2011Perspective: Big and LittleFall 2011 SymposiumSpring 2012 PlansWith International Experience: Ireland What Honors Continues to Do for Me Stay Connected
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Inside this Issue: Community Garden and Relay for LifeSouthern Regional Honors Council ConferenceCongratulations May 2011 Graduates!Why I Teach HonorsWUHA! - A Semester in PicturesNew WUHA! OfficersReflection on Spring 2011Fall 2011 PlansHonors Educational Experiences Student Spotlight: Amy RiversStudy Abroad
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Inside this Issue: WUHA! Can Drive and Rollin’ in Rock HillWhy I Chose Honors… What Honors Has Done for Me...The OfficeCongrats GradWhy I Teach HonorsWUHA! - A Semester in PicturesSpring 2011 PlansFall 2010 ReflectionHonors Symposia SRHC and KIVAStudy Abroad and NSE
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Inside this Issue: Relay for Life KivaWhy I Chose Honors… What Honors Has Done for Me...Congratulations, May 2010 GraduatesWUHA!, - A Semester in PicturesWelcome, Class of 2014!Honors Symposia SRHCStudy Abroad: South Africa and Ireland
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Inside this Issue: Service Learning HighlightsCongratulations, December Graduate!WUHA! - A Semester in PicturesHonors SymposiaNCHCStudy AbroadWhere Are Honors Freshmen From?
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Inside this Issue: WUHA! Service Learning HighlightsSouthern Regional Honors Council ConferenceHonors Program GraduatesHonorable MentionsCongratulations, Dr. DisneyWith International ExperienceFall 2009 Calendar and Events
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Display of work accomplished by Section 4 and 9 of the 2005 Foundation students. Index to student work filed with the poster.
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A resistência a doenças em plantas transgênicas tem sido obtida por meio da expressão de genes isolados de bactérias, fungos micoparasitas e plantas. Neste trabalho, relatamos a utilização de um gene do fungo entomopatogênico Metarhizium anisopliae como modo de gerar resistência a doenças fúngicas em plantas. O gene chit1 codifica a quitinase CHIT42 (EC 3.2.1.14), pertencente a uma classe de glicosil-hidrolases capazes de converter quitina em oligômeros de N-acetil-glicosamina (NAcGlc). Quando presentes em tecidos vegetais, supõese que as quitinases ataquem especificamente a parede celular de fungos invasores, provocando danos às hifas e causando a morte por lise das células fúngicas. Deste modo, dois diferentes grupos de plantas transgênicas de Nicotiana tabacum foram produzidos: no primeiro deles, denominado chitplus, os indivíduos possuem o gene chit1 sob o controle do promotor CaMV 35S. O segundo grupo, demoninado chitless, consiste de plantas transformadas com um T-DNA não contendo o gene do fungo. Trinta e quatro plantas transgênicas resistentes à canamicina (17 de cada grupo) foram regeneradas a partir de discos de folhas infectados por Agrobacterium tumefaciens. A produção da quitinase em extratos protéicos de folhas foi analisada por zimogramas em SDS-PAGE contendo glicol-quitina e corados por calcoflúor branco, na forma de um screening dos transgênicos primários. As plantas transgênicas foram testadas, ainda, por meio de ensaios colorimétricos empregando oligômeros sintéticos de NAcGlc como substratos específicos, além de immunoblot e Western blot com soro anti-quitinase. A quantidade de enzima recombinante nas plantas chitplus variou desde nenhuma atividade detectável a elevados níveis de expressão da enzima. A hibridização de Southern blot demonstrou que o número de cópias do gene chit1 integradas no genoma vegetal foi estimado entre uma e quatro. A primeira geração de plantas transgênicas geradas por autofecundação de parentais portadores de duas cópias do transgene foi testada com relação à estabilidade da herança do transgene e em 43 de um total de 67 descendentes, originados de quatro cruzamentos independentes, o padrão de segregação não diferiu das proporções Mendelianas esperadas. Ensaios de resistência, desafiando as plantas transgênicas com o basidiomiceto Rhizoctonia solani foram realizados e uma evidente diminuição da área foliar contendo lesões fúngicas foi observada entre as linhagens transgênicas, embora variações na atividade quitinolítica tenham influenciado o nível de resistência. Nossos resultados sugerem uma relação direta entre a atividade específica de quitinase e ao aumento nos níveis de resistência às lesões causadas pela infecção por R. solani.
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Companies have looked for many new ways to communicate with their customers. In the current scenario, Facebook has proven to be an efficient communication tool between consumers and businesses. This study aims to understand the differences in the complaint messages sent to companies, through an experiment that measured the emotional tone and the lack of formality in each message received by the website and the Facebook page of the company. As expected, people are more informal on Facebook. However, contrary to our intuition, participants tended to display more emotions on the company website. The social norms theory and the impression management contributed to explain the phenomena found.
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-D-glucosidase (EC 3.2.1.21) is one of the most interesting glycosidases, especially for hydrolysis cellobiose releasing glucose, is last step degradation of cellulose. This function makes the -D-glucosidase is of great interest as a versatile industrial biocatalyst, being critical to various bio-treatment / biorefinery processes, such as bioethanol production. Hen in the report, a -D-glucosidase was extracts from protein extracted of the invertebrate marine Artemia franciscana was purified and characterized with a combination of precipitation with ammonium sulfate (0 - 30%, 30 to 50%, 50 to 80%), the fraction saturated in the range of 30 to 50% (called F-II) was applied in a molecular exclusion chromatography, in Sephacryl S-200, the fractions corresponding to the first peak of activity of -D-glucosidase were gathered and applied in a chromatography of ion exchange in Mono Q; the third peak this protein obtained chromatography, which coincides with the peak of activity of -D-glucosidase was held and applied in a gel filtration chromatography Superose 12 where the first peak protein, which has activity of -D-glucosidase was rechromatography on Superose 12. This enzyme is probably multimerica, consisting of three subunit molecular mass of 52.7 kDa (determined by SDS-PAGE) with native molecular mass of 157 kDa (determined by gel filtration chromatography on Superose 12 under the system FPLC). The enzyme was purified 44.09 times with a recovery of 1.01%. Using up p-nitrophenyl-β-D-glucopiranoside as substrate obtained a Km apparent of 0.229 mM and a Vmax of 1.109 mM.60min-1.mL-1mM. The optimum pH and optimum temperature of catalysis of the synthetic substrate were 5.0 and 45 °C, respectively. The activity of the -D-glucosidase was strongly, inhibited by silver nitrate and N- etylmaleimide, this inhibition indicates the involvement of radical sulfidrila the hydrolysis of synthetic substrate. The -D-glucosidase of Artemia franciscana presented degradativa action on celobiose, lactose and on the synthetic substrate -nitrophenyl-β-D-glucopiranoside indicating potential use of this enzyme in the industry mainly for the production of bioethanol (production of alcohol from the participating cellulose), and production hydrolysate milk (devoid of milk lactose)
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Lectin obtained from the marine sponge Tedania ignis was purified and characterized by extraction of soluble proteins (crude extract) in 50mM Borax, pH 7.5. The purification procedure was carried out by crude extract precipitation with ammonium sulfate 30% (FI). The precipitated was resuspended in the same buffer and fractionated with acetone 1.0 volume (F1.0). A lectin was purified from this specific fraction by using an affinity chromatography Sepharose 6B. This lectin preferentially agglutinated human erythrocytes from B type previously treated with papain enzyme. The hemagglutinating activity lectin was dependent of divalent Mn2+ cation and was inhibited by the carbohydrates galactose, xylose and fructose. SDS-PAGE analysis indicated a molecular mass of the lectin around 45 kDa. This protein showed stability until 40°C for 1 h. Further, it showed activity between pH 2.5 and 11.5, with an enhanced activity at pH 7.5. Leishmania chagasi promastigotes stained with Coomassie brilliant blue R-250 were agglutinated by F1,0 and in the presence of galactose this interaction was abolished. These results show that this lectin could be implicated in defense procedures and it will can be used as biological tools in studies with this protozoon
