Crystal Structures of a Bacterial Isocitrate Dehydrogenase and the Human Sulfamidase / Pushing the Limits of Molecular Replacement

Sidhu, Navdeep Singh

09 January 2014

No description available.

540

sulfamidase

crystal structure

isocitrate dehydrogenase

molecular replacement

sulfamate sulfohydrolase

heparan N-sulfatase

N-sulfoglucosamine sulfohydrolase

Chemie  (PPN62138352X)

Evaluation of method for function control of test assay’s complementing and signaling enzymes

Strand, Alva

January 2022

Nucleoside 5'-Diphosphate Kinase (NdPK EC 2.7.4.6) is an enzyme (phosphotransferase) with extraordinary characteristics due to its unique ability to transfer phosphor groups to interconvert all nucleoside di- and triphosphates as a part of the DNA synthesis. Due to Biovica International AB's use of signaling and complementing enzymes in their in vitro diagnostic (IVD) test assays for Thymidine Kinase activity, an investigation was proposed to evaluate NdPK, which is a complementing enzyme in the assay. The aim of the study was to evaluate the enzymatic turnover of the enzyme NdPK with a spectrophotometric assay to obtain the specific activity (Units/mg solid protein). To determine the specific activity, enzyme kinetic methodology was applied, including the Michaelis-Menten model. In this study, the method is proposed as a general internal control procedure for the company, as a tool for function control of the different purchased enzymes used in their products in development. Results from the study reflects the different methods used to gain the specific activity for NdPK, where they were compared with the already specified specific activity from the manufacturing company. The results were auspicious, but before the method's authorization as an internal quality procedure, a few amendments are in mind. For instance, determining a method for the graphical readings, validating the method for quality control, and investigating if the method is applicable to other complementing enzymes. In conclusion, the method for determining the specific activity of the enzyme NdPK can be done, by executing the procedure of colorimetric enzyme assay.

Nucleoside 5´-Diphosphate Kinase (NdPK)

Adenosine 5´-Triphosphate (ATP)

Rate-limiting enzyme

Enzymatic specific activity.

Biomedical Laboratory Science/Technology

Transient State Monitoring and Fluorescence Correlation Spectroscopy of Flavin Adenine Dinucleotide

Egnell, Liv

January 2014

Many human diseases including cancer have been associated with altered cellular metabolism and a changed oxygen consumption in cells. Fluorophores are sensitive to their local environment due to their long life times in transient dark states. A recent study successfully utilized this sensitivity to image differences in oxygen concentrations in cells using transient state (TRAST) microscopy together with fluorescent labels [1]. A natural continuation of this study is to investigate the possibilities of using this method with natural fluorophores already present in cells and thereby avoid articial labeling. Flavin adenine dinucleotide (FAD) is an auto fluorescent coenzyme that is naturally present in cells and involved in cellular metabolism. This project is an exploratory pilot study for cellular measurements with the aim to investigate if FAD can be used to probe oxygen concentrations in aqueous solution using transient state monitoring and fluorescence correlation spectroscopy (FCS). This thesis includes the results from FCS and TRAST experiments on FAD in aqueous solutions with different oxygen concentrations as well as different ascorbic acid concentrations. The performed experiments showed that FAD monitored with TRAST is sensitive to differences in oxygen concentrations for the aqueous solutions used in this study.

Transient State Monitoring

Fluorescence Correlation Spectroscopy

Flavin Adenine Dinucleotide

FCS

TRAST

FAD

Biophysics

Biofysik

Engineering and Technology

Teknik och teknologier

Medical Engineering

Medicinteknik

Two-pore channels and NAADP-dependent calcium signalling

Calcraft, Peter James

January 2010

Nicotinic acid adenine dinucleotide phosphate (NAADP) is a potent Ca²⁺ mobilising messenger in mammalian and non-mammalian cells. Studies on a variety of cell types suggest that NAADP evokes Ca²⁺ release from a lysosome-related store and via activation of a receptor distinct from either ryanodine receptors (RyR) or inositol 1,4,5-trisphosphate (IP₃) receptors (IP₃R). However, the identity of the NAADP receptor has, until now, remained elusive. In this thesis I have shown that NAADP-evoked Ca²⁺ release from lysosomes is underpinned by two-pore channels (TPCs), of which there are 3 subtypes, TPC1, TPC2 and TPC3. When stably over-expressed in HEK293 cells, TPC2 was found to be specifically targeted to lysosomes, while TPC1 and TPC3 were targeted to endosomes. Initial Ca²⁺ signals via TPC2, but not those via TPC1, were amplified into global Ca²⁺ waves by Ca²⁺-induced Ca²⁺ release (CICR) from the endoplasmic reticulum (ER) via IP₃Rs. I have shown that, consistent with a role for TPCs in NAADP-mediated Ca²⁺ release, TPC2 is expressed in pulmonary arterial smooth muscle cells (PASMCs), is likely targeted to lysosomal membranes, and that TPCs also underpin NAADP-evoked Ca²⁺ signalling in this cell type. However, and in contrast to HEK293 cells, in PASMCs NAADP evokes spatially restricted Ca²⁺ bursts that are amplified into global Ca²⁺ waves by CICR from the sarcoplasmic reticulum (SR) via a subpopulation of RyRs, but not via IP₃Rs. I have demonstrated that lysosomes preferentially co-localise with RyR subtype 3 (RyR3) in the perinuclear region of PASMCs to comprise a “trigger zone” for Ca²⁺ signalling by NAADP, away from which a propagating Ca²⁺ wave may be carried by subsequent recruitment of RyR2. The identification of TPCs as a family of NAADP receptors may further our understanding of the mechanisms that confer the versatility of Ca²⁺ signalling which is required to regulate such diverse cellular functions as gene expression, fertilization, cell growth, and ultimately cell death.

572

Caracterização molecular e morfológica de populações de Aedes aegypti (Diptera:Culicidae) no estado de São Paulo. / Molecular and morphological characterization of Aedes aegypti populations (Diptera: Culicidae) from State of São Paulo.

Vidal, Paloma Oliveira

17 November 2015

O Estado de São Paulo apresenta uma das mais altas taxas de infecções por vírus dengue no Mundo, mas apesar dessa situação, poucos são os estudos dirigidos às populações do mosquito Aedes aegypti. O objetivo deste trabalho foi caracterizar geneticamente e morfologicamente populações de Ae. aegypti localizadas em seis municípios (Santos, S.P., Campinas, São Carlos, Catanduva, S.J.R.P.) do Estado de São Paulo durante 2011 e 2012. Todos os marcadores biológicos indicaram estruturação populacional. Os oito loci microssatélites apontaram diferenciação genética moderada entre as populações (Fst= 0.04; p < 0,05) e os níveis de diversidade nucleotídica do gene COI (&pi; =0,0062) e do gene ND4 (&pi;=0,017) foram moderadamente altos. Duas linhagens geneticamente distintas foram encontradas no Estado. Ao longo dos meses que compreenderam o estudo, foram encontradas diferenças morfo-genéticas temporais entre as seis populações analisadas, possivelmente indicativas de microevolução. Os resultados obtidos podem ser úteis para compreendermos a dispersão deste mosquito vetor. / The State of São Paulo displays one of the highest rates of dengue infection in the world, but despite this fact, a few populational studies of Ae. aegypti have been undertaken. The aim of this study was to genetically and morphologically characterize Ae. aegypti populations from six locations in the São Paulo State (Santos, S.P., Campinas, São Carlos, Catanduva, S.J.R.P.) during 2011 and 2012. The phenetic and genetic analyses revealed that populations of Ae. aegypti are structured. Eight microsatellites loci were polymorphic and genetic differentiation among samples was moderate (Fst= 0.04; p < 0.05). Nucleotide diversities of COI (&pi; = 0.0062) and ND4 gene (&pi; = 0.017) were moderately high. Two lineages distinct genetically were found in the State. Over the months comprised by the study, we found the temporal genetics and morphologics differences among the six populations, a possibly indicative of microevolution of mosquitoes. The results of this study may be useful for understand the spread of this vector mosquitoes in the State of São Paulo.

Citocromo oxidase subunidade I

COI

COI

Culicidae

Culicídeos

Cytochrome oxidase subunit I

Microevolução

Microevolution

Microsatellites

Microssatélites

Morfometria geométrica alar

Mosquitoes

Mosquitos

ND4

ND4

Wing geometric morphometrics

Kinetic behavior of the NAD(P)H:Quinone oxidoreductase WrbA from Escherichia coli. / Kinetic behavior of the NAD(P)H:Quinone oxidoreductase WrbA from Escherichia coli.

KISHKO, Iryna

January 2012

This Ph.D. thesis addresses the structure-function relationship of the multimeric oxidoreductase WrbA with the principal aim being the explanation of the unusual kinetics of this enzyme in molecular terms, and thus getting an insight about its physiological role in bacteria. WrbA is a multimeric enzyme with FMN as a co-factor, catalyzing the oxidation of NADH by a two electrons transfer. Structure and function analysis of WrbA places this enzyme between bacterial flavodoxins and eukaryotic oxidoreductases in terms of its evolutionary relationship. The kinetic activity of WrbA was studied under varying conditions such as temperature, pH etc, and its kinetic mechanism was evaluated from parameters KM and Vmax and confirmed by product inhibition pattern experiments. Crystallization and proteolytic experiments also underpin the functional importance of the multimeric nature of WrbA and aid the understanding of the physiological role of this enzyme in molecular terms.

Structural bioinformatics tools for the comparison and classification of protein interactions

Garma, L. D. (Leonardo D.)

08 August 2017

Abstract Most proteins carry out their functions through interactions with other molecules. Thus, proteins taking part in similar interactions are likely to carry out related functions. One way to determine whether two proteins do take part in similar interactions is by quantifying the likeness of their structures. This work focuses on the development of methods for the comparison of protein-protein and protein-ligand interactions, as well as their application to structure-based classification schemes. A method based on the MultiMer-align (or MM-align) program was developed and used to compare all known dimeric protein complexes. The results of the comparison demonstrates that the method improves over MM-align in a significant number of cases. The data was employed to classify the complexes, resulting in 1,761 different protein-protein interaction types. Through a statistical model, the number of existing protein-protein interaction types in nature was estimated at around 4,000. The model allowed the establishment of a relationship between the number of quaternary families (sequence-based groups of protein-protein complexes) and quaternary folds (structure-based groups). The interactions between proteins and small organic ligands were studied using sequence-independent methodologies. A new method was introduced to test three similarity metrics. The best of these metrics was subsequently employed, together with five other existing methodologies, to conduct an all-to-all comparison of all the known protein-FAD (Flavin-Adenine Dinucleotide) complexes. The results demonstrates that the new methodology captures the best the similarities between complexes in terms of protein-ligand contacts. Based on the all-to-all comparison, the protein-FAD complexes were subsequently separated into 237 groups. In the majority of cases, the classification divided the complexes according to their annotated function. Using a graph-based description of the FAD-binding sites, each group could be further characterized and uniquely described. The study demonstrates that the newly developed methods are superior to the existing ones. The results indicate that both the known protein-protein and the protein-FAD interactions can be classified into a reduced number of types and that in general terms these classifications are consistent with the proteins' functions. / Tiivistelmä Suurin osa proteiinien toiminnasta tapahtuu vuorovaikutuksessa muiden molekyylien kanssa. Proteiinit, jotka osallistuvat samanlaisiin vuorovaikutuksiin todennäköisesti toimivat samalla tavalla. Kahden proteiinin todennäköisyys esiintyä samanlaisissa vuorovaikutustilanteissa voidaan määrittää tutkimalla niiden rakenteellista samankaltaisuutta. Tämä väitöskirjatyö käsittelee proteiini-proteiini- ja proteiini-ligandi -vuorovaikutusten vertailuun käytettyjen menetelmien kehitystä, ja niiden soveltamista rakenteeseen perustuvissa luokittelujärjestelmissä. Tunnettuja dimeerisiä proteiinikomplekseja tutkittiin uudella MultiMer-align-ohjelmaan (MM-align) perustuvalla menetelmällä. Vertailun tulokset osoittavat, että uusi menetelmä suoriutui MM-alignia paremmin merkittävässä osassa tapauksista. Tuloksia käytettiin myös kompleksien luokitteluun, jonka tuloksena oli 1761 erilaista proteiinien välistä vuorovaikutustyyppiä. Luonnossa esiintyvien proteiinien välisten vuorovaikutusten määrän arvioitiin tilastollisen mallin avulla olevan noin 4000. Tilastollisen mallin avulla saatiin vertailtua sekä sekvenssin (”quaternary families”) sekä rakenteen (”quaternary folds”) mukaan ryhmiteltyjen proteiinikompleksien määriä. Proteiinien ja pienien orgaanisten ligandien välisiä vuorovaikutuksia tutkittiin sekvenssistä riippumattomilla menetelmillä. Uudella menetelmällä testattiin kolmea eri samankaltaisuutta mittaavaa metriikkaa. Näistä parasta käytettiin viiden muun tunnetun menetelmän kanssa vertailemaan kaikkia tunnettuja proteiini-FAD (Flavin-Adenine-Dinucleotide, flaviiniadeniinidinukleotidi) -komplekseja. Proteiini-ligandikontaktien osalta uusi menetelmä kuvasi kompleksien samankaltaisuutta muita menetelmiä paremmin. Vertailun tuloksia hyödyntäen proteiini-FAD-kompleksit luokiteltiin edelleen 237 ryhmään. Suurimmassa osassa tapauksista luokittelujärjestelmä oli onnistunut jakamaan kompleksit ryhmiin niiden toiminnallisuuden mukaisesti. Ryhmät voitiin määritellä yksikäsitteisesti kuvaamalla FAD:n sitoutumispaikka graafisesti. Väitöskirjatyö osoittaa, että siinä kehitetyt menetelmät ovat parempia kuin aikaisemmin käytetyt menetelmät. Tulokset osoittavat, että sekä proteiinien väliset että proteiini-FAD -vuorovaikutukset voidaan luokitella rajattuun määrään vuorovaikutustyyppejä ja yleisesti luokittelu on yhtenevä proteiinien toiminnan suhteen.

binding site comparison

flavin adenine dinucleotide (FAD)

protein-protein interactions

structural alignment

structural bioinformatics

structural similarity

flaviiniadeniinidinukleotidi (FAD)

proteiini-proteiini vuorovaikutus

rakenteellinen samankaltaisuus

rakenteeseen perustuva bioinformatiikka

rakenteiden rinnastus

sitoutumispaikkavertailu

Effects of Nicotinamide Riboside and Beta-hydroxybutyrate on C. elegans Lifespan

Peters, Jeffery

01 May 2020

The nicotinamide riboside (NR) form of vitamin B3and the ketone body ß-hydroxybutyrate (BHB) are two of the most promising natural compounds yet identified for the treatment of aging and aging-related diseases. Forms of vitamin B3are precursors for the synthesis of the coenzymes nicotinamide adenine dinucleotide (NAD(H)) and nicotinamide adenine dinucleotide phosphate (NADP(H)). In aged cells levels of NAD+decline, decreasing metabolism and decreasing activity of protective sirtuin protein deacetylases. In aged cells NR, but not more common forms of vitamin B3, boost NAD+levels. BHB is naturally produced by the body when individuals fast or consume a ketogenic (KD) or calorically restricted (CR) diet. These diets have been shown to extend lifespan in mice, while they are also protective in many disease models. Caenorhabditis elegans, a roundworm with a short mean lifespan of roughly 2 to 3 weeks depending upon the temperature, is used as a model system to study aging. BHB has been previously shown to increase lifespan by roughly 20% when administered to C. elegans.We administered NR and BHB individually and together to C. elegans starting at two different developmental stages (larval stages 1 and 4) and measured lifespan. We found that administration of 20 mM DL-BHB decreased lifespan when first given at the L1 stage, while it robustly increased lifespan when first given at the L4 stage. Administration of 0.5 mM NR increased lifespan when first given at L1, with only a very slight increase when first given at L4. When initiating administration at L1, NR greatly mitigated the BHB-mediated decline in longevity, however, NR did not increase BHB-mediated lifespan extension when first administered at L4.

Lifespan

C. elegans

Nicotinamide Riboside

Beta-hydroxybutyrate

Ketogenic Diet

Nicotinamide Adenine Dinucleotide

Biochemistry

Chemical Actions and Uses

Genetic Phenomena

Medical Biochemistry

Medical Cell Biology

Medical Physiology

Organic Chemicals

Development and Characterization of an Iridium-Modified Electrochemical Biosensor for Potential Diabetic Patient Management

Fang, Lei

January 2009

No description available.

Biochemistry

Biomedical Research

Chemical Engineering

Engineering

Iridium-modified

Electrochemical biosensor

Think film printing

Diabetic patient management

Ketone body

3-hydroxybutyrate(3HB)

Nicotinamide adenine dinucleotide(NAD+)

Glycosylated hemoglobin (HbA1c)

Fructosyl valine

Diffusion-reaction model

The Rtg1 and Rtg3 proteins are novel transcription factors regulated by the yeast hog1 mapk upon osmotic stress

Noriega Esteban, Núria

27 February 2009

La adaptación de la levadura Saccharomyces cerevisiae a condiciones de alta osmolaridad está mediada por la vía de HOG ((high-osmolarity glycerol). La activación de esta vía induce una serie de respuestas que van a permitir la supervivencia celular en respuesta a estrés. La regulación génica constituye una respuesta clave para dicha supervivencia. Se han descrito cinco factores de transcripción regulados por Hog1 en respuesta a estrés osmótico. Sin embargo, éstos no pueden explicar la totalidad de los genes regulados por la MAPK Hog1. En el presente trabajo describimos cómo el complejo transcripcional formado por las proteínas Rtg1 y Rtg3 regula, a través de la quinasa Hog1, la expresión de un conjunto específico de genes. Hog1 fosforila Rtg1 y Rtg3, aunque ninguna de estas fosforilaciones son esenciales para regulación transcripcional en respuesta a estrés. Este trabajo también muestra cómo la deleción de proteínas RTG provoca osmosensibilidad celular, lo que indica que la integridad de la vía de RTG es esencial para la supervivencia celular frente a un estrés osmótico. / In Saccharomyces cerevisiae the adaptation to high osmolarity is mediated by the HOG (high-osmolarity glycerol) pathway, which elicits different cellular responses required for cell survival upon osmostress. Regulation of gene expression is a major adaptative response required for cell survival in response to osmotic stress. At least five transcription factors have been reported to be controlled by the Hog1 MAPK. However, they cannot account for the regulation of all of the genes under the control of the Hog1 MAPK. Here we show that the Rtg1/3 transcriptional complex regulates the expression of specific genes upon osmostress in a Hog1-dependent manner. Hog1 phosphorylates both Rtg1 and Rtg3 proteins. However, none of these phosphorylations are essential for the transcriptional regulation upon osmostress. Here we also show that the deletion of RTG proteins leads to osmosensitivity at high osmolarity, suggesting that the RTG-pathway integrity is essential for cell survival upon stress.

OD: optical density

NAD+: nicotinamide adenine dinucleotide

MAPK: mitogen activated protein kinase

HOG: high osmolarity glycerol

ERC: extrachromosomal rDNA circles

CDK: cyclin dependent kinase

DNA: desoxirribobucleic acid

ATP: adenosine triphosphate

AMP: adenosine monophosphate

TOR: Diana de la rapamicina

STRE element de resposta a l'estrés

ROS: especies reactives de l'oygen

rDNA: DNA risbosomal

OD: densitat òptica

NAD+: nicotinàmida adenina dinucleòtid

HOG: osmolaritat elevada de glicerol

rDNA: risbosomal DNA

ERC: cercle d'rDNA extracromosòmic

DNA: àcid desoxirriblonucleic

CDK: Kinassa dependent de ciclines

ATP: trifosfat d'adenosina

AMP: monofosfat d'adenosina

ROS: reactive oxygen species

SAPK: stress activated protein kinase

STRE: stress response element

TOR: target of rapamycin

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