Molecular and Genetic Strategies to Enhance Functional Expression of Recombinant Protein in Escherichia coli

Narayanan, Niju

January 2009

The versatile Escherichia coli facilitates protein expression with relative simplicity, high cell density on inexpensive substrates, well known genetics, variety of expression vectors, mutant strains, co-overexpression technology, extracytoplasmic secretion systems, and recombinant protein fusion partners. Although, the protocol is rather simple for soluble proteins, heterologous protein expression is frequently encountered by major technical limitations including inefficient translation, formation of insoluble inclusion bodies, lack of posttranslational modification mechanisms, degradation by host proteases, and impaired cell physiology due to host/protein toxicity, in achieving functional expression of stable, soluble, and bioactive protein.. In this thesis, model protein expression systems are used to address the technical issues for enhancing recombinant protein expression in E. coli. When yellow fluorescence protein (YFP) was displayed on E. coli cell surface, the integrity of the cell envelope was compromised and cell physiology was severely impaired, resulting in poor display performance, which was restored by the coexpression of Skp, a periplasmic chaperone. On the basis of monitoring the promoter activities of degP, rpoH, and cpxP under various culture conditions, it was demonstrated that the cell-surface display induced the σE extracytoplasmic stress response, and PdegP::lacZ was proposed to be a suitable “sensor” for monitoring extracytoplasmic stress. Intracellular proteolysis has been recognized as one of the key factors limiting recombinant protein production, particularly for eukaryotic proteins heterologously expressed in the prokaryotic expression systems of E. coli. Two amino acids, Leu149 and Val223, were identified as proteolytically sensitive when Pseudozyma antarctica lipase (PalB) was heterologously expressed in Escherichia coli. The functional expression was enhanced using the double mutant for cultivation. However, the recombinant protein production was still limited by PalB misfolding, which was resolved by DsbA coexpression. The study offers an alternative genetic strategy in molecular manipulation to enhance recombinant protein production in E. coli. To overcome the technical limitations of protein misfolding, ineffective disulfide bond formation, and protein instability associated with intracellular proteolysis in the functional expression of recombinant Pseudozyma antarctica lipase B (PalB) in Escherichia coli, an alternative approach was explored by extracellular secretion of PalB via two Sec-independent secretion systems, i.e. the α-hemolysin (Type I) and the modified flagellar (Type III) secretion systems, which can export proteins of interest from the cytoplasm directly to the exterior of the cell. Bioactive PalB was expressed and secreted extracellularly either as HlyA fusion (i.e. PalB-HlyA via Type I system) or an intact protein (via Type III system) with minimum impact on cell physiology. However, the secretion intermediates in the intracellular fraction of culture samples were non-bioactive even though they were soluble, suggesting that the extracellular secretion did mediate the development of PalB activity. PalB secretion via Type I system was fast with higher specific PalB activities but poor cell growth. On the other hand, the secretion via Type III system was slow with lower specific PalB activities but effective cell growth. Functional expression of lipase from Burkholderia sp. C20 (Lip) in various cellular compartments of Escherichia coli was explored. The poor expression in the cytoplasm was improved by several strategies, including coexpression of the cytoplasmic chaperone GroEL/ES, using a mutant E. coli host strain with an oxidative cytoplasm, and protein fusion technology. Fusing Lip with the N-terminal peptide tags of T7PK, DsbA, and DsbC was effective in boosting the solubility and biological activity. Non-fused Lip or Lip fusions heterologously expressed in the periplasm formed insoluble aggregates with a minimum activity. Biologically active and intact Lip was obtained upon the secretion into the extracellular medium using the native signal peptide and the expression performance was further improved by coexpression of the periplasmic chaperon Skp. The extracellular expression was even more effective when Lip was secreted as a Lip-HlyA fusion via the α-hemolysin transporter. Finally, Lip could be functionally displayed on the E. coli cell surface when fused with the carrier EstA.

Escherichia coli

recombinant protein expression

cell-surface display

protein secretion

inclusion bodies

proteolysis

mutagenesis

chaperone

fusion tags

cell physiology

stress pathways

Chemical Engineering

Strategies for facilitated production of recombinant proteins in escherichia coli

Hedhammar, My

January 2005

<p>The successful genomic era has resulted in a great demand for efficient production and purification of proteins. The main objective of the work described in this thesis was to develop methods to facilitate recovery of target proteins after recombinant production in Escherichia coli.</p><p>A positively charged purification tag, Z_basic, has previously been constructed by protein design of a compact three-helix bundle domain, Z. The charged domain was investigated for general use as a fusion partner. All target proteins investigated could be selectively captured by ion-exchange chromatography under conditions excluding adsorption of the majority of Escherichia coli host proteins. A single cation-exchange chromatography step at physiological pH was sufficient to provide Z_basic fusion proteins of high purity close to homogeneity. Moreover, efficient isolation directly from unclarified <i>Escherichia coli</i> homogenates could also be accomplished using an expanded bed mode. Since the intended use of a recombinant protein sometimes requires removal of the purification tag, a strategy for efficient release of the Z_basic moiety using an immobilised protease was developed. The protease columns were reusable without any measurable decrease in activity. Moreover, subsequent removal of the released tag, Z_basic, was effected by adsorption to a second cation-exchanger. </p><p>Using a similar strategy, a purification tag with a negatively charged surface, denoted Z_acid, was constructed and thoroughly characterised. Contrary to Z_basic, the negatively charged Z_acid was highly unstructured in a low conductivity environment. Despite this, all Z_acid fusion proteins investigated could be efficiently purified from whole cell lysates using anion-exchange chromatography</p><p>Synthesis of polypeptides occurs readily in Escherichia coli providing large amounts of protein in cells of this type, albeit often one finds the recombinant proteins sequestered in inclusion bodies. Therefore, a high throughput method for screening of protein expression was developed. Levels of both soluble and precipitated protein could simultaneously be assessed <i>in vivo</i> by the use of a flow cytometer. </p><p>The positively charged domain, Z_basic, was shown also to be selective under denaturing conditions, providing the possibility to purify proteins solubilised from inclusion bodies. Finally, a flexible process for solid-phase refolding was developed, using Z_basic as a reversible linker to the cation-exchanger resin.</p>

ion-exchange chromatography

protein A

Z

Zbasic

Zacid

fusion protein

proteolytic cleavage

immobilised protease

flow cytometry

inclusion bodies

solid-phase refolding

Molecular biology

Molekylärbiologi

<i>Cauliflower mosaic virus</i> Inclusion Body Formation: The Where, The How and The Why

Alers-Velazquez, Roberto M.

January 2020

No description available.

Molecular Biology

Virology

LifeAct

Latrunculin B

GFP250

Liquid-liquid phase separation

Nonmembranous organelles

Pararetrovirus

Particle tracking

qPCR

DAS-ELISA

CaMV

P6

inclusion bodies

Talin

symptom formation

temperature

Méthodes de production et étude électrophysiologique de canaux ioniques : application à la pannexine1 humaine et au canal mécanosensible bactérien MscL / Production methods and electrophysiological study of ion channels : application to the human pannexine 1 and to the bacterial mechanosensitive channel MscL.

Assal, Reda

14 December 2011

La production hétérologue des protéines membranaires reste difficile, peut-être parce que l’insertion dans la membrane de la cellule hôte constitue une étape limitante de la production. Afin de tourner cette difficulté, deux modes de synthèse ont été envisagés: la synthèse de protéines dans un système a-cellulaire, en l’absence de membrane mais en présence de détergent, ou l’adressage forcé de la protéine vers les corps d’inclusion dans le cas d’une expression plus classique en bactérie entière. La réalisation des deux stratégies repose sur l’utilisation de protéines de fusion possédant une séquence d’entraînement en amont du gène d’intérêt, soit qu’elles améliorent la traduction du transcrit en limitant le repliement spatial de ce dernier, soit qu’elles favorisent la production de la protéine d’intérêt en corps d’inclusion. La porine OmpX et le peptide T7 ont été choisis en cas d’expression dans les systèmes bactériens. La protéine SUMO est utilisée pour la production dans un lysat eucaryote. Les différentes approches ont été testées sur la production de la pannexine1 humaine (Px1).Si les séquences d’entraînement OmpX et le peptide T7 sont correctement produites in vitro, aucune des deux, en revanche, ne favorise la production de la Px1. Seul l’entraîneur SUMO est efficace. En effet, nous avons observé que cette protéine augmente la production de la Px1 dans un lysat eucaryote de germe de blé. Par ailleurs OmpX, connue pour être largement produite in vivo dans les corps d’inclusion, n’entraîne pas la localisation de la Px1 dans ces structures. Contre toute attente, l’étiquette T7 dirige la Px1 dans les corps d’inclusion. L’étude électrophysiologique de la Px1 a donc été effectuée à partir de la protéine produite in vivo (T7his-Px1) après renaturation, ou produite sous forme soluble in vitro (his6-Px1) dans le lysat eucaryote. Dans le cas de la protéine T7his-Px1 renaturée, une activité canal qui rappelle celle qui est observée après expression dans l’ovocyte de Xénope, a été détectée en patch-clamp, mais dans trois cas seulement. Dans le cas de la protéine his6-Px1, aucune activité canal n’est clairement détectée. Dans une deuxième partie de ce travail on examine le rôle de la boucle périplasmique dans la sensibilité à la pression du MscL, un canal mécanosensible bactérien devenu un système modèle dans l’étude de la mécanosensibilité. Presque toutes les études fonctionnelles sur ce canal ont été réalisées sur le canal de E.coli, alors que la structure a été obtenue à partir de l’homologue de M. tuberculosis. Une étude fonctionnelle a montré que le MscL de M. tuberculosis est difficile à ouvrir : son ouverture requiert l’application d’une pression double de celle qui est nécessaire chez E.coli. Les deux homologues diffèrent principalement par la longueur de leur unique boucle périplasmique. De manière à examiner le rôle de la boucle, on a comparé l’activité du canal MscL de E.coli, celle du canal de M. tuberculosis et celle d’une protéine chimère constituée de la protéine de M. tuberculosis dans laquelle la boucle a été changée pour celle de la protéine de E.coli. De manière inattendue, nous avons constaté que les canaux de E.coli et de M. tuberculosis ont la même sensibilité à la pression. La protéine chimère n’avait pas d’activité canal. Si ce travail ne permet pas de conclure quant au rôle de la boucle, il montre sans ambigüité que contrairement à ce qui a été rapporté les canaux MscL de E.coli et de M. tuberculosis ne diffèrent pas sensiblement sur le plan fonctionnel / The production of heterologous membrane protein is notoriously difficult; this might be due to the fact that insertion of the protein in the membrane host is a limiting step. To by-pass this difficulty, two modes of synthesis were tested: 1) production in a cell-free system devoid of biological membrane but supplemented with detergent or liposomes, 2) production in bacteria, with targeting of the membrane protein to inclusion bodies. Both strategies were tested for the production of the human pannexin 1 channel (Px1). The gene coding the protein was fused with an “enhancer” sequence resulting in the addition of a peptide or short protein at the N terminus of the protein of interest. This enhancer sequence which is well produced in vitro or in vivo is supposed to facilitate the translation of the protein of interest. Three enhancer sequences were chosen: 1) the small porin OmpX of E. coli, which, in addition, should target the protein to inclusion bodies when the protein is expressed in bacteria 2) a peptide of phage T7 for expression in E.coli lysate or E.coli cells 3) the small protein SUMO for production in a wheat germ cell-free system. In a bacterial cell-free system, neither OmpX nor T7 promoted Px1 production. Px1 is only produced when the SUMO enhancer sequence is used in the wheat germ system. In bacteria, OmpX, known to form inclusions bodies did not promote the targeting of the fusion protein to inclusion bodies. Unexpectedly, the peptide T7 was able to do it.Px1 obtained from inclusion bodies (T7his-Px1) was renatured and reconstituted in liposomes. Similarly his6-Px1 produced in wheat germ system was reconstituted in liposomes. Both preparations were used for electrophysiological studies (patch-clamp and planar bilayers). With the refolded T7his-Px1, channel activity reminiscent of that observed with Px1 expressed in Xenope oocyte (Bao et al., 2004) could be detected, but only in three cases. In the case of his6-Px1, no clear channel activity could be observed. The second part of this work deals with the involvement of the periplasmic loop of the bacterial mechanosensitive channel MscL in its sensitivity to pressure. Mscl has become a model system for the investigation of mechanosensisity. Nearly all functional studies have been performed on MscL from E.coli while the structure of the protein has been obtained from the Mycobacterium tuberculosis homologue. In one functional study it was shown that MscL from M. tuberculosis is extremely difficult to open, gating at twice the pressure needed for E.coli MscL The periplasmic loop is the most variable sequence between the two homologues, being longer in E.coli than in M. tuberculosis. In order to assess the role of the periplamic loop in the sensitivity to pressure, we compared the activity of the E.coli and M. tuberculosis MscL and of a chimeric protein made of the M. tuberculosis protein in which the periplasmic loop has been exchanged for that of the E. coli channel. Unexpectedly, M. tuberculosis and E .coli MscL were observed to gate at a similar applied pressure. The chimeric protein had no functional activity. In conclusion, this study does not allow any conclusion as to the role of the loop in the sensitivity to pressure, but it shows clearly that, in contrast to the results of a previous study, there is no functional difference between E. coli and M. tuberculosis MscL.

Protéines membranaires

Synthèse acellulaire

Corps d'inclusion

Séquences d'entrainement

Peptide T7

Porine OmpX

Canaux ioniques

Canaux mécanosensibles

MscL

Pannexine

Electrophysiologie

Patch-clamp

BLM

Membrane protein production

Cell-free system

Inclusion bodies

Ion channel

Mechanosensitive channel

MscL

Pannexin

Electrophysiology

Patch-clamp

BLM

Expression, solubilisation, purification and characterisation of recombinant bluetongue virus viral protein 7

Russell, Bonnie Leigh

10 1900

Bluetongue virus belongs to the Orbivirus genus from the Reoviridae family. It infects predominantly domestic and wild ruminants and is economically significant worldwide. Bluetongue virus VP7 forms the intercepting layer between the outer capsid (VP2 and VP5) and VP3 which surrounds the genomic material. BL21(DE3), NiCo21(DE3), C43(DE3) pLysS and KRX Escherichia coli cells were transformed with a pET28a plasmid with the cDNA sequence encoding Bluetongue virus VP7. Expression of Bluetongue virus VP7 was tested at post induction temperatures between 16˚C and 37 ˚C, at inducer concentrations between 0.1 mM and 1.0 mM isopropyl-β-D-thiogalactopyranoside in BL21(DE3), NiCo21(DE3) and C43(DE3) pLysS cells and 0.05 % and 0.15 % rhamnose for KRX cells, in two types of growth media (LB and 2xYT) and post-induction growth times between two and 16 hours. Under all conditions tested; Bluetongue virus VP7 expression was found to be predominantly in the insoluble fraction (pellet). BL21(DE3) and NiCo21(DE3) cells were chosen and grown for five hours post induction, induced with 0.1 mM isopropyl-β-D-thiogalactopyranoside and grown at a post-induction temperature of 37 ˚C. Bluetongue virus VP7 in bacterial cell inclusion bodies was solubilised using urea and a freeze-thaw step. Solubilisation was tested with urea concentrations between 2 M and 8 M, with solubilisation efficiency not increasing past 5 M urea. Solubilized Bluetongue virus VP7 was purified using nickel-affinity chromatography. Purified Bluetongue virus VP7 was then probed with far-UV circular dichroism and intrinsic fluorescence in several buffer conditions including different urea and guanidinium chloride concentrations as well as in the presence of glycerol and sodium chloride. Guanidinium chloride was able to cause Bluetongue virus VP7 unfolding, and the unfolding transition had 94 % and 89 % reversibility at 218 nm and 222 nm respectively. Bluetongue virus VP7 was shown to contain a native-like structure in 20 % glycerol and in up to 8 M urea and was found to be stable till at least 55 ˚C, even in the presence of 5 M urea. Glycerol and sodium chloride influenced the conformation of the protein resulting in different unfolding transitions. Thermal unfolding of Bluetongue virus VP7 was found to be irreversible. / Life and Consumer Sciences / M. Sc. (Life Sciences)

Bluetongue virus

Escherichia coli

Far-UV circular dichroism

Fluorescence

Inclusion bodies

Polyhistidine-tagged purification

Protein expression

Protein solubilisation

Protein stability

VP7

636.3089691

Solubilization

Recombinant proteins

Bluetongue virus

Viral proteins

Escherichia coli

Fluorescence

Sheep -- Virus diseases

Sicherheitsforschung und Monitoringmethoden zum Anbau von Bt-Mais: Expression, Nachweis und Wirkung von rekombinantem Cry1Ab in heterologen Expressionssystemen / Biosafety research and monitoring methods of Bt-corn: Expression, detection and effect of recombinant Cry1Ab in heterologous expression systems

Nguyen, Thu Hang

08 November 2004

No description available.

570 Biowissenschaften

Biologie

Agricultural Sciences

Bacillus thuringiensis

Cry1Ab-Protoxin

aktives Cry1Ab-Toxin

Proteineinschlusskörper

Trypsinisierung

Maiszünsler

Ostrinia nubilalis

Biotest

LC50

Toxizität

Antikörper

ELISA

immunologischer Nachweis

Bt-Mais

Expression

Toxingehalt.

Bacillus thuringiensis

Cry1Ab-protoxin

active Cry1Ab-toxin

protein inclusion bodies

trypsinization

European corn borer

Ostrinia nubilalis

Bioassay

LC50

toxicity

antibody

ELISA

immunological detection

Bt-corn

expression

toxin level.

48.00

42.20

WF

WR

WW