Produção de proteínas recombinantes em células BHK-21 cultivadas em meio livre de soro fetal bovino. / Production of recombinant proteins in BHK-21 cells cultured in serum free media.

Patiño, Sandra Fernanda Suárez

06 May 2016

Células eucariotas usadas como plataforma de expressão de proteínas recombinantes são geralmente cultivadas com soro fetal bovino (SFB), porém, abordagens biotecnológicas atuais sobre cultura de células devem evitar o uso deste suplemento, devido a problemas de custo, variações entre os lotes e risco de contaminação. Assim, nosso objetivo foi expressar as proteínas recombinantes: GFP (proteína verde fluorescente), NS3 (proteína não estrutural 3 do vírus da hepatite C) e RVGP (glicoproteína do vírus da raiva) em células BHK-21 adaptadas em meios livres de soro fetal bovino (SFM) usando o sistema de expressão baseado no Semliki Forest Virus (SFV). Os resultados do presente trabalho mostraram que células adaptadas em SFM cresceram de forma eficiente, produziram mais partículas virais recombinantes de SFV do que células suplementadas com soro, sendo que estas partículas virais podem ser usadas diretamente para imunização, pois garantiram uma amplificação e expressão eficiente das diferentes proteínas dentro da célula hospedeira. / Eukaryotic cells are cultured with serum, however current biotechnological approaches of cell culture need to avoid using of this supplement, due to the high costs, lot-to-lot variation and risk of contamination. Thus, our aim was to express the recombinant protein: GFP (green fluorescent protein); NS3 (Hepatitis C virus non-structural protein 3) and RVGP (rabies virus glycoprotein) in BHK-21 cells cultured in serum free culture based on Semliki Forest Virus system. The results of this work showed that cells cultured in serum-free media (SFM) were grown efficiently, they were produce more recombinant viral particles when compared with cells supplemented with SFB. These viral particles can be used directly for immunization, since generated amplification and expression efficient of different proteins within the host cell.

Semliki Forest Virus

BHK-21 cells

Células BHK-21

Fetal bovine serum

Glicoproteína do vírus da raiva

Green fluorescent protein

Meio livre de soro

Proteína verde fluorescente

Rabies virus glycoprotein

Semliki Forest Virus

Serum-free medium

Soro fetal bovino-SFB

New insights in photodynamic theraphy: production, diffusion and reactivity of singlet oxygen in biological systems

Jiménez Banzo, Ana María

25 April 2008

S'ha estudiat la cinètica de fotosensibilització de l'oxigen singlet (1O2) en cèl·lules eucariotes en suspensió mitjançant un espectròmetre d'última generació amb resolució temporal per sota del microsegon. Els estudis revelen que la cinètica del 1O2 depèn del seu lloc de formació. Per una banda, la producció del 1O2 es més lenta en els lisosomes que en el nucli. Per altra banda, el 1O2 es capaç d'escapar de les cèl·lules quan es fotosensibilitza en el nucli, però es queda confinat al interior si es fotosensibilitza en els lisosomes. Malgrat que el temps de vida del 1O2 es troba en els microsegons, la desactivació principal ve donada per interaccions amb les biomolècules característiques de cadascú dels orgànuls. La incertesa respecte a la producció de 1O2 en un orgànul determinat es pot eliminar mitjançant l'ús de fotosensibilitzadors modificats genèticament, ja que aquets poden ésser expressats selectivament. Amb aquesta finalitat, s'avaluen les propietats fotosensibilitzants de mutants de proteïna fluorescent verd (GFP). Algunes de les GFPs estudiades sensibilitzen la formació del 1O2 malgrat amb baixa eficiència. Els resultats obtinguts es comparen amb els del cromòfor de la GFP i mostren que l'estructura proteínica, a sobre de modular les propietats fotofísiques del cromòfor, també el protegeix de la desactivació col·lisional. Finalment, s'estudien les propietats d'absorció bifotónica del 2,7,12,17-tetrafenilporficé i del seu complex de pal·ladi (II). L'eficiència de formació del 1O2 per part dels dos compostos, desprès de l'absorció simultània de dos fotons, es aproximadament 100 vegades superior a la dels seus anàlegs porfirínics, amb seccions d'absorció bifotòniques δ ~ 25 GM. Les excel·lents propietats d'aquestos compostos s'expliquen mitjançant arguments qualitatius i s'analitzen les seves perspectives de cara al seu ús en teràpia fotodinámica. / Se ha estudiado la cinética de fotosensibilización de 1O2 en células eucariotas en suspensión, usando un espectrómetro de última generación con resolución temporal por debajo del microsegundo. Los estudios revelan que la cinética del 1O2 depende de su lugar de formación. Por una parte, la producción de 1O2 es más lenta en los lisosomas que en el núcleo. Por otra parte, el 1O2 es capaz de escapar de las células cuando es fotosensibilizado en el núcleo, mientras que queda confinado en el interior si se fotosensibiliza en los lisosomas. A pesar de que el tiempo de vida del 1O2 se encuentra en los microsegundos, la desactivación principal viene dada por interacciones con las biomoléculas características de cada orgánulo. La incertidumbre respecto a la producción de 1O2 en un orgánulo determinado puede ser eliminada mediante el uso de fotosensibilizadores modificados genéticamente ya que pueden ser expresados selectivamente. Con este fin, se evalúan las propiedades fotosensibilizantes de mutantes de proteína fluorescente verde (GFP). Algunas de las GFPs estudiadas sensibilizan la formación de 1O2 aunque con baja eficiencia. Los resultados obtenidos se comparan con los del cromóforo de la GFP y muestran que la estructura proteínica, además de modular las propiedades fotofísicas del cromofóro, también lo protege de la desactivación colisional. Finalmente, se estudian las propiedades de absorción bifotónica del 2,7,12,17-tetrafenilporficeno y de su complejo de paladio (II). La eficacia de formación de 1O2 de ambos compuestos, tras la absorción simultánea de dos fotones, es aproximadamente 100 veces superior a la de sus análogos porfirínicos, con secciones de absorción bifotónica δ ~ 25 GM. Las excelentes propiedades de estos compuestos se explican mediante argumentos cualitativos y se analizan sus perspectivas de cara a su uso en terapia fotodinámica. / The kinetics of singlet oxygen (1O2) photosensitisation in human skin fibroblasts have been investigated by means of an ultrasensitive near-infrared spectrometer with submicrosecond time resolution. The results indicate that the 1O2 kinetics are site-dependent. On one hand, the production of 1O2 is slower in the lysosomes than in the nucleus. On the other hand, 1O2 is able to escape out of the cells when photosensitised in the nucleus, while 1O2 photosensitized in the lysosomes is confined. Despite showing a lifetime in the microsecond time domain, the decay of 1O2 is governed by interactions with the biomolecules within the organelle there it is produced. The uncertainty as to the intracellular site of 1O2 production may be removed by the use of genetically-encoded photosensitisers, which can be expressed in any desired organelle. Towards this end, the ability of some fluorescent proteins (GFPs) to photosensitise 1O2 has been studied. Some of the studied proteins are able to produce 1O2 albeit with a very low quantum yield. The results obtained are compared to those of the synthetic GFP chromophore and indicates that the protein scaffold not only plays a role in modulating the photophysical properties of the chromophore but also has a protective function from collisional quenching. Finally, the two-photon absorption properties of tetraphenylporphycene and its palladium (II) complex have been determined. These compounds are ca. 100-fold more efficient two-photon 1O2 photosensitisers than their isomeric porphyrin counterparts, with two-photon absorption cross sections δ ~ 25 GM. Qualitative symmetry-based arguments are provided to explain the excellent two-photon properties and the prospects for photodynamic therapy are discussed.

two-photon

time-resolved

subcellular localisation

singlet oxygen

porphycene

photosensitiser

photodynamic therapy

fibroblasts

Green Fluorescent Protein

kinetics

diffusion

terapia fotodinámica

resolución temporal

porficeno

proteína fluorescente verde

localización subcelular

oxígeno singlete

fotosensibilizador

fibroblastos

bifotónico

difusión

cinética

teràpia fotodinàmica

fotosensibilitzador

localització subcel·lular

oxigen singlet

porficè

proteïna fluorescent verd

resolució temporal

fibroblasts

difusió

bifotònic

cinètica

Química i Enginyeria Química

544

Generation of Novel Photochromic GFPs: Fluorescent Probes for RESOLFT-type Microscopy at Low Light Intensities / Entwicklung neuartiger photochromer GFPs: fluoreszente Marker für die RESOLFT-basierte Mikroskopie bei geringen Lichtintensitäten

Grotjohann, Tim

18 April 2012

No description available.

570 Biowissenschaften, Biologie

WA 310

Biology (incl. Psychology)

RESOLFT

rsEGFP

RSFP

STED

rsEGFP2

Fluoreszenzmikroskopie

hochauflösende Mikroskopie

EGFP

RESOLFT

rsEGFP

RSFP

STED

rsEGFP2

fluorescence microscopy

superresolution microscopy

EGFP

42.03

Ultraschnelle, lichtinduzierte Primärprozesse im elektronisch angeregten Zustand des Grün Fluoreszierenden Proteins (GFP) / Ultrafast Elementary Events in the Excited State of Green Fluorescent Protein (GFP)

Winkler, Kathrin

24 January 2003

No description available.

540 Chemie

Mathematics and Computer Science

Grün Fluoreszierendes Protein (GFP)

Pump-Probe-Spektroskopie

Protonentransfer

ultraschnell

innere Konversion

Schwingungsenergietransfer

Green Fluorescent Protein (GFP)

pump-probe-spectroscopy

excited state proton transfer

ultrafast

internal conversion

vibrational energy transfer

35.13

35.25

35.16

SIL 000: Laser-Chemie {Strahlungschemie}

SGF 400

RRQ 000: Laser-Spektroskopie {Physik}

WCE 000: Photobiologie {Biophysik}

Funktionelle Rekonstitution von Connexonen in artifizielle Membranen: Expression, Reinigung und Charakterisierung von Connexin 43 / Functional reconstitution of connexons in artificial membranes: expression, purification and characterization of connexin 43

Carnarius, Christian

11 June 2012

No description available.

570 Biowissenschaften

Biologie

SX 000

WC 000

WR 000

SXH 000

Chemistry

Connexin 43

Cx43

Grün fluoreszierendes Protein

GFP

Porenüberspannende Membranen

Poröses Aluminiumoxid

Artifizielle Membranen

Planar Patch Clamp

Melittin

Pichia pastoris

D. discoideum

connexin 43

Cx43

green fluorescent protein

GFP

pore spanning membranes

porous alumina

artificial membranes

planar patch clamp

melittin

Pichia pastoris

Dictyostelium discoideum

42.12

35.78

35.71

Produção de proteínas recombinantes em células BHK-21 cultivadas em meio livre de soro fetal bovino. / Production of recombinant proteins in BHK-21 cells cultured in serum free media.

Sandra Fernanda Suárez Patiño

06 May 2016

Células eucariotas usadas como plataforma de expressão de proteínas recombinantes são geralmente cultivadas com soro fetal bovino (SFB), porém, abordagens biotecnológicas atuais sobre cultura de células devem evitar o uso deste suplemento, devido a problemas de custo, variações entre os lotes e risco de contaminação. Assim, nosso objetivo foi expressar as proteínas recombinantes: GFP (proteína verde fluorescente), NS3 (proteína não estrutural 3 do vírus da hepatite C) e RVGP (glicoproteína do vírus da raiva) em células BHK-21 adaptadas em meios livres de soro fetal bovino (SFM) usando o sistema de expressão baseado no Semliki Forest Virus (SFV). Os resultados do presente trabalho mostraram que células adaptadas em SFM cresceram de forma eficiente, produziram mais partículas virais recombinantes de SFV do que células suplementadas com soro, sendo que estas partículas virais podem ser usadas diretamente para imunização, pois garantiram uma amplificação e expressão eficiente das diferentes proteínas dentro da célula hospedeira. / Eukaryotic cells are cultured with serum, however current biotechnological approaches of cell culture need to avoid using of this supplement, due to the high costs, lot-to-lot variation and risk of contamination. Thus, our aim was to express the recombinant protein: GFP (green fluorescent protein); NS3 (Hepatitis C virus non-structural protein 3) and RVGP (rabies virus glycoprotein) in BHK-21 cells cultured in serum free culture based on Semliki Forest Virus system. The results of this work showed that cells cultured in serum-free media (SFM) were grown efficiently, they were produce more recombinant viral particles when compared with cells supplemented with SFB. These viral particles can be used directly for immunization, since generated amplification and expression efficient of different proteins within the host cell.

Semliki Forest Virus

Células BHK-21

Glicoproteína do vírus da raiva

Meio livre de soro

Proteína verde fluorescente

Soro fetal bovino-SFB

BHK-21 cells

Fetal bovine serum

Green fluorescent protein

Rabies virus glycoprotein

Semliki Forest Virus

Serum-free medium

Lineage tracing of Ascl1-expressing cells in the maternal liver during pregnancy

Nambiar, Shashank Manohar

January 2014

Indiana University-Purdue University Indianapolis (IUPUI) / To cope with the high metabolic demands of the body during pregnancy, the maternal liver adapts by increasing its mass and size. This increase is proportional to the increase in total body weight during the course of gestation. The pregnancy-induced maternal liver growth is a result of both hepatocyte hypertrophy and hyperplasia. Microarray analysis of pregnant maternal livers shows markedly different gene expression profiles when compared to a non-pregnant state. Most interesting was the 2,500-fold up-regulation in the mRNA expression of Ascl1, a transcription factor responsible for the differentiation of neural progenitor cells into various neuronal types, during the second half of pregnancy. Our investigation aimed at (1) characterizing the identity of maternal hepatic Ascl1-expressing cells and (2) tracing the fate of Ascl1-expressing cells in the maternal liver during pregnancy. Timed pregnancies were generated and non-pregnant (NP) and pregnant maternal livers were harvested and analysed. To identify the maternal hepatic Ascl1-expressing cells we used the Ascl1GFP/+ reporter mouse line. NP and gestation day 15 (D15) maternal livers were immunostained for green fluorescent protein (GFP). The result shows that GFP-positive, Ascl1-expressing cells are hepatocyte-like cells, which are present in D15 maternal livers, but absent in NP livers. The Rosa26floxstopLacZ/ floxstopLacZ;Ascl1CreERT2/+ mouse line was used to trace the fate of Ascl1-expressing cells during pregnancy. LacZ staining of gestation day 13 (D13) and 18 (D18) maternal livers demonstrates that D13 hepatic Ascl1-expressing cells (labeled with LacZ) undergo hyperplasia to repopulate a large portion of D18 maternal livers. Furthermore, LacZ and HNF4α co-staining of D13 and D18 maternal livers shows the presence of two populations of LacZ-expressing cells: HNF4α+ population and HNF4α- population. HNF4α+ LacZ-expressing cells represent hepatocyte lineage cells that are derived from Ascl1-expressing cells. We observe that, towards the end of pregnancy, a considerable portion of the maternal liver is comprised of hepatocytes derived from Ascl1-expressing cells. Taken together, our preliminary study suggests that pregnancy induces maternal liver turnover via Ascl1-expressing cells.

Liver -- Growth -- Research

Hyperplasia -- Research

Gene expression -- Research

Pregnancy -- Research

Liver -- Regeneration

Neural stem cells -- Research

Messenger RNA

Stem cells -- Research

Animal models in research

Veranschaulichung subzellulärer physikalischer Kräfte biochemischen und mechanischen Ursprungs mittels FRET / Insights into the spatiotemporal regulation of the cellular cytoskeleton through applications of FRET

Mitkovski, Miso

03 November 2005

No description available.

570 Biowissenschaften, Biologie

Mathematics and Computer Science

förster resonanz energie transfer

FRET

biosensor

design

optischer kraft-biosensor

dipol orientation

optimierung

kraftausübung

zelladhesion

Rho GTPase

fluoreszenz aktivierte zell-sortierung

extrazelluläre matrix

EZM

grün fluoreszierendes protein

gfp

cfp

venus

förster resonance eneregy transfer

FRET

biosensor

design

optical force biosensor

dipole orientation

optimization

force exertion

cell adhesion

Rho GTPase

fluorescence activated cell sorting

FACS

extracellular matrix

ECM

green fluorescent protein

gfp

cfp

venus

42.03

42.12

42.13

42.15

WCE 000: Photobiologie {Biophysik}

WA 310: Mikroskopie {Biologie}

WA 320: Spektroskopie {Biologie}

Mecanismes de regulació en l'activitat biològica del factor de transcripció Snail

Domínguez Solà, David

03 April 2003

Els factors de transcripció de la família Snail són fonamentals en la "transició epiteli-mesènquima", procés morfogènic essencial en el desenvolupament embrionari i en els fenòmens metastàsics tumorals.En els mamífers l'activitat d'Snail és modulada per dos mecanismes. (i) En el promotor humà es troben regions definides de resposta a factors repressors, predominants en les cèl·lules epitelials, i elements diferenciats de resposta a inductors de la "transició epiteli-mesènquima". (ii) L'activitat d'Snail és condicionada també per la seva localització subcel·lular, modulada per mecanismes no transcripcionals: la fosforilació d'Snail determina si és o no exclós del nucli. Al citosol no pot actuar com a repressor transcripcional però pot interaccionar amb la xarxa microtubular, que estabilitza i en condiciona el dinamisme. Això coincideix amb l'activació de la GTPasa RhoA i la reorientació dels filaments de vimentina, fets associats a l'adquisició de capacitat migratòria. L'efecte com a repressor transcripcional i la modulació del dinamisme microtubular són possiblement esdeveniments coordinats necessaris per al rol biològic d'Snail en mamífers. / Snail family of transcription factors is fundamental to the "epithelial-mesenchymal transition", morphogenic process essential to embryonic development and metastatic phenomena in tumors.Snail's activity is modulated in two ways in mammals. (i) The human promoter harbors definite regions that respond to repressor factors, which prevail in epithelial cells; and differentiated elements that respond to known inducers of the "epithelial-mesenchymal transition". (ii) Snail's activity is also conditioned by its subcellular localization, mechanism not dependent on its transcriptional control: Snail phosphorylation determines whether Snail is excluded or not from the nucleus. When in the cytosol, Snail is unable to act as a transcriptional repressor, but however binds to the microtubular meshwork, which becomes stabilized and whose dynamism is conditioned as a result. This fact coincides with the activation of the RhoA GTPase and reorientation of vimentin filaments, both phenomena being related to the acquisition of cell motility. The transcriptional repressor and the microtubule dynamics effects are probably two coordinated events necessary to Snail's biological role in mammals.

Polimerització in vitro

PKCzeta

PKC atípica (Protein Kinase C)

P65

Promotor

Nocodazol

NF-kB/Dorsal (Nuclear Factor Kappa-B)

NES (seqüència d'export nuclear)

Microtúbuls detirosinats

Microtúbuls

Metàstasi

Invasió

Adenocarcinoma

ARNm

Beta-catenina

Centrosoma

CLIP-170

Cancer

Cresta neural

CRM1 (Chromosome Region Maintenance 1)

Despolimerització microtúbuls

Dit de Zenc atípic

Dit de Zenc

Domini ric en Serines

Ebox

E-cadherina

Espais intercromatínics

Estabilització microtúbuls

Export nuclear

Filaments intermediaris

Fosforilació

Gastrulació

GFP (Green Fluorescent Protein)

Heterocarions

ILK (Integrin Linked Kinase)

Promotor

Reconstrucció fronts invasius

Regulació

Retrogen

RhoA

GTPasa

SC35

Slug

SNAG (domini)

SNAI1L

Snail

Speckles nuclears

Time-lapse

Èster de forbol

Transició Epiteli-Mesènquima

Transcripció / Transcripcional

U2AF65

Vimentina

57

Orthogonality and Codon Preference of the Pyrrolysyl-tRNA Synthetase-tRNAPyl pair in Escherichia coli for the Genetic Code Expansion

Odoi, Keturah

2012 May 1900

Systematic studies of basal nonsense suppression, orthogonality of tRNAPyl variants, and cross recognition between codons and tRNA anticodons are reported. E. coli displays detectable basal amber and opal suppression but shows a negligible ochre suppression. Although detectable, basal amber suppression is fully inhibited when a pyrrolysyl-tRNA synthetase (PylRS)-tRNAPyl_CUA pair is genetically encoded. trnaPyl_CUA is aminoacylated by an E. coli aminoacyl-tRNA synthetase at a low level, however, this misaminoacylation is fully inhibited when both PylRS and its substrate are present. Besides that it is fully orthogonal in E. coli and can be coupled with PylRS to genetically incorporate a NAA at an ochre codon, tRNAPyl_UUA is not able to recognize an UAG codon to induce amber suppression. This observation is in direct conflict with the wobble base pair hypothesis and enables using an evolved M. jannaschii tyrosyl-tRNA synthetase-tRNAPyl_UUA pair and the wild type or evolved PylRS-tRNAPyl_UUA pair to genetically incorporate two different NAAs at amber and ochre codons. tRNAPyl_UCA is charged by E. coli tryptophanyl-tRNA synthetase, thus not orthogonal in E. coli. Mutagenic studies of trnaPyl_UCA led to the discovery of its G73U form which shows a higher orthogonality. Mutating trnaPyl_CUA to trnaPyl_UCCU not only leads to the loss of the relative orthogonality of tRNAPyl in E. coli but also abolishes its aminoacylation by PylRS.

Pyl, pyrrolysine

PylRS, pyrrolysyl-tRNA synthetase

NAA, noncanonical amino acid

aaRS, aminoacyl-tRNA synthetase

T4 PNK, T4 polynucleotide kinase

AzF, para-azido-L-phenylalanine

PCR, polymerase chain reaction

RF, release factor

TrpRS, tryptophanyl-tRNA synthetase

ArgRS, arginyl-tRNA synthetase

Trp, tryptophan

Lys, lysine

Glu, glutamate

Gln, glutamine

Phe, phenylalanine

Arg, arginine.