Expression of Arabidopsis thaliana cellulose synthase proteins and associated proteins in a Spodoptera frugiperda cell line

Lyons, Jessy

01 October 2012

Understanding how cellulose synthesis occurs is key to understanding the formation of the plant cell wall. This understanding could also be key to modifying cellulose production to permit more efficient extraction of glucose from cellulose for the production of biobased materials. Cellulose biosynthesis is carried out by cellulose synthases; transmembrane multimeric processive glycosyltransferases responsible for polymerizing UDP‐glucose into glucan chains. Thirty‐six glucan chains bind together in parallel to form elementary cellulose microfibrils. Due to the essential nature of cellulose synthases for plant survival and the recalcitrant nature of the cell wall to chemical and enzymatic digestion, the cellulose synthases can be very difficult to analyze by traditional approaches. In an attempt to circumvent some of the issues of studying cellulose synthases, the cellulose synthase genes CESA1 and CESA3, along with the cell wall associated genes COBRA, DET3 and POM1 were recombined into an engineered Autographa californica nucleopolyhedron virus and expressed in Spodoptera fruigiperda ovarian cells. Although recombinant protein could be detected for CESA1 and CESA3, C14‐glucose incorporation on baculovirus infected cell lines have given inconclusive results to the cellulose synthase activity of the CESA1 and CESA3 proteins. With further optimization of the protein expression of CESA1 and optimization of the variability in the C14‐glucose incorporation assays, the baculovirus system may prove a useful tool for studying the cellulose synthases. / UOIT

Arabidopsis

Cellulose synthase

SF9

DET3

Purification and Uptake Studies of Recombinant Human N-α-D-Acetylglucosaminidase from Sf9 Insect Cells

Morris, Geoffrey

27 August 2015

Human α-N-acetylglucosaminidase (Naglu) is a lysosomal enzyme implicated in the rare metabolic storage disorder Mucopolysaccharidosis III type B (MPS IIIB). A deficiency in Naglu results in a buildup of heparan sulfate in lysosomes, which is most detrimental in the central nervous system, causing mental retardation and a shortened lifespan. Enzyme replacement therapy is currently ineffective in treating the neurological symptoms of MPS IIIB due to the inability of Naglu to cross the blood-brain barrier. This laboratory uses a Spodoptera frugiperda insect cell system to express recombinant Naglu conjugated to a synthetic protein transduction domain with the intent to allow Naglu to cross the blood-brain barrier and treat the neurological symptoms. In the present study, we aimed to purify a recombinant Naglu-PTD4 fusion protein in order to assess its capacity to cross cellular membranes. A three-step method involving multi-modal, hydrophobic interaction, and gel filtration chromatography was optimized to achieve pure Naglu-PTD4, in good yield. Cellular uptake by human MPSIIIB fibroblasts of Naglu-PTD4 was not detectable. It is hypothesized that additional amino acids, including a hexahistidine domain, following the PTD4 domain limited the fusion protein’s membrane transduction capacity. Future studies will focus on removing the additional amino acids and adjusting the purification method as necessary. The ultimate goal of this research is to develop a large-scale recombinant Naglu production protocol for enzyme replacement therapy of MPS IIIB. / Graduate

Naglu

Protein Purification

Sf9

Sanfilippo Syndrome B

MPS IIIB

Cellular Uptake

FPLC

Mapping the Conformational Dynamics of E-selectin upon Interaction with its Ligands

Aleisa, Fajr A

15 May 2013

Selectins are key adhesion molecules responsible for initiating a multistep process that leads a cell out of the blood circulation and into a tissue or organ. The adhesion of cells (expressing ligands) to the endothelium (expressing the selectin i.e.,E-selectin) occurs through spatio-temporally regulated interactions that are mediated by multiple intra- and inter-cellular components. The mechanism of cell adhesion is investigated primarily using ensemble-based experiments, which provides indirect information about how individual molecules work in such a complex system. Recent developments in single-molecule (SM) fluorescence detection allow for the visualization of individual molecules with a good spatio-temporal resolution nanometer spatial resolution and millisecond time resolution). Furthermore, advanced SM fluorescence techniques such as Förster Resonance Energy Transfer (FRET) and super-resolution microscopy provide unique opportunities to obtain information about nanometer-scale conformational dynamics of proteins as well as nano-scale architectures of biological samples. Therefore, the state-of-the-art SM techniques are powerful tools for investigating complex biological system such as the mechanism of cell adhesion. In this project, several constructs of fluorescently labeled E-selectin will be used to study the conformational dynamics of E-selectin binding to its ligand(s) using SM-FRET and combination of SM-FRET and force microscopy. These studies will be beneficial to fully understand the mechanistic details of cell adhesion and migration of cells using the established model system of hematopoietic stem cells (HSCs) adhesion to the selectin expressing endothelial cells (such as the E-selectin expressing endothelial cells in the bone marrow).

E-Selectin

cloning

Sf9 cells

CHO-Kl cells

Hermatopoietic stem cells (HSC)

Forster resonance energy transfer (FRET)

Rat protease-activated receptor–1 (rPAR1) expression and characterization in Sf9 cells

Lavalle, Maria

07 1900

Connue pour son rôle dans la cascade de coagulation, la thrombine, une protéase à sérine, peut également agir par l’intermédiaire de PAR1, un récepteur activé par protéase et couplé aux protéines G liant le GTP (GPCR). La thrombine se lie et clive l’extrémité N-terminale du PAR1 entre l’Arg41 et la Ser42, exposant une nouvelle extrémité terminale qui agit elle-même comme un ligand. La thrombine et une séquence peptidique de cinq acides aminés, composée des résidus Ser42 à Arg46, nommée PAR1-AP, déclenchent dans diverses cellules de mammifères une réponse intracellulaire comportant une composante calcique. Dans cette étude, le système d’expression par baculovirus dans les cellules Sf9 d'insecte nous a permis d'exprimer le récepteur PAR1 du rat à la surface de ces cellules et de réaliser son couplage fonctionnel à leur signalisation intracellulaire (modèle rPAR1-Sf9). La composante calcique de celle-ci, en réponse au PAR1-AP, a ensuite été étudiée en détail à l’aide de la sonde fluorescente Fura-2 et de plusieurs inhibiteurs agissant sur les canaux calciques ou d'autres éléments de la cascade de signalisation du calcium intracellulaire. Lorsque le milieu extracellulaire contient du calcium (Ca2+), la thrombine ou PAR1-AP déclenchent un signal calcique qui consiste en une augmentation rapide de [Ca2+]i suivi d’un plateau relativement soutenu, puis d'un retour lent vers le niveau de base initial. En l'absence de Ca2+ dans le milieu extracellulaire, l'augmentation initiale rapide de [Ca2+]i est suivie d'un retour rapide vers le [Ca2+]i de base. À l’aide d’inhibiteurs de canaux calciques, tels que le lanthane, la nifédipine et le D-600, l'entrée du calcium du milieu extracellulaire dans les cellules est inhibée, abolissant le plateau soutenu de [Ca2+]i. L’inhibition de la pompe Ca2+-ATPase par la thapsigargine supprime la réponse au PAR1-AP après épuisement des sites de stockage de Ca2+intracellulaire. Le TMB-8 agit de façon discordante quant à l’inhibition de la libération de Ca2+ des sites de stockage intracellulaires. La réponse à PAR1-AP n’est pas affectée par le D-609, un inhibiteur de la phospholipase β. L’inhibition de la protéine kinase C (PKC) par le bisindolylmaléimide induit des oscillations en présence de Ca2+ extracellulaire et atténue fortement le signal calcique en absence de Ca2+ extracellulaire. En présence de Ca2+ extracellulaire, l’activation de la PKC par le PBDu tronque le flux de [Ca2+]i tandis que la réponse calcique est abolie en absence de Ca2+ dans le milieu extracellulaire. Le H-89, un inhibiteur de la protéine kinase A (PKA), cause une prolongation de la durée du plateau de [Ca2+]i dans un milieu riche en calcium et la suppression de la réponse à PAR1-AP lorsque le milieu extracellulaire est dépourvu de Ca2+. Les résultats obtenus nous permettent de conclure que la PKC et possiblement la PKA jouent un rôle critique dans la mobilisation du Ca2+ induite par le PAR1-AP dans le modèle rPAR1-Sf9. / Thrombin’s serine protease activity allows for it to have a role in both the coagulation cascade as well as through a GTP- binding protein coupled receptor (GPCR) known as the protease-activated receptor-1 (PAR1). Thrombin binds to PAR1 at the N-terminal, cleaving between Arg41 and Ser42, and unmasking a new N-terminal which acts as a tethered ligand. Thrombin and a five amino acid peptide composed of the sequence of residues Ser42 to Arg46, known as PAR 1-AP, has been shown to mediate a number of signalling mechanisms in mammalian cells, including a calcium signalling pathway. In the present study, the Sf9-baculovirus system allowed us to express the rat PAR1 (rPAR1-Sf9) on the cell surface and study its intracellular signalling. The calcium (Ca2+) signal was studied using the fluorescent probe Fura-2, and several Ca2+ channel inhibitors and calcium signal modulators were used to study the signal induced by PAR1-AP. In the presence of extracellular calcium [Ca2+]e, thrombin and PAR1-AP produced a Ca2+ signal which consisted of an initial spike in [Ca2+]i followed by a relatively maintained plateau and a slow return towards baseline. In the absence of Ca2+ in the extracellular space, the initial Ca2+ increase is followed by a quick return to baseline [Ca2+]i. Ca2+ channel inhibitors, lanthanum, nifedipine and D-600, inhibited the entry of Ca2+ from the extracellular space and abolished the plateau phase of the response to PAR1-AP. Inhibition of the Ca2+-ATPase with thapsigargin abolished the response to PAR1-AP after having depleted the Ca2+ stores involved in the initial spike in [Ca2+]i. TMB-8, expected to inhibit the release of Ca2+ from internal stores, inconsistently inhibited the [Ca2+]i response to PAR1-AP. The response elicited by PAR1-AP was not affected by D-609, an inhibitor of phospholipase Cβ. Inhibition of protein kinase C (PKC) with bisindolylmaleimide induced oscillations in the [Ca2+]i levels in the presence of extracellular Ca2+ while it significantly blunted the response in the absence of extracellular Ca2+. PDBu activation of PKC truncated the [Ca2+]i surge in Ca2+-rich conditions while abolishing it altogether in the absence of extracellular Ca2+. H-89 inhibition of protein kinase A (PKA) prolonged the plateau duration in Ca2+-rich medium while inhibiting the response to PAR1-AP in a Ca2+-deficient environment. Taken together, our results suggest that PKC and possibly PKA play a critical role in the mobilisation of Ca2+ in rPAR1-Sf9 by PAR1-AP.

Cellule Sf9

baculovirus

thrombine

récepteur activé par protéase

signalisation calcique

canal calcique

Fura-2

thrombin

protease-activated receptor

calcium channel

calcium signalling

Sf9 cell

Regulation of productivity in Trichoplusia ni and Spodoptera frugiperda Sf9 serum-free cultures

Calles, Karin

January 2005

<p>The aim of this work has been to characterize the effects of conditioned medium (CM) on insect cell productivity and physiology in order to get a better understanding about the mechanisms that regulate productivity in serum-free media. Two cell lines have been investigated, Spodoptera frugiperda (Sf9) and Trichoplusia ni (T. ni, BTI-Tn-5B1-4). The baculovirus expression vector system (BEVS) was used for protein expression, using the ligand-binding domain of the human glucocorticoid receptor as a model protein. Addition of CM at inoculation led to a shorter lag phase and that the cells reached the maximum cell density faster than cells in fresh medium for both Sf9 and T. ni cells. Sf9 cells passed a switch in growth kinetics after 30-40 passages. At this point, CM lost its stimulating effect on proliferation. CM also affected the cell size and cell cycle progression. Sf9 and T. ni cells became smaller when CM was added at inoculation because they had a minor arrest in the cell cycle after inoculation and therefore started to divide earlier than cells in fresh medium. For Sf9 cells, this was illustrated by a smaller arrest in G2/M in the beginning of culture and the cells were consequently less synchronized. For T. ni cells, the initial decrease in the S phase population was followed by an earlier increase of the S phase population for the cells with CM than for the cells in fresh medium.</p><p>Addition of 20 % CM or CM filtrated with a 10 kDa cut-off filter to Sf9 cultures had a negative effect on the specific productivity. However, addition of CM to Sf9 cells that had passed the switch in growth kinetics had no negative effect on productivity. This indicates that CM not affects the protein production per se, but rather through its effects on cell physiology. Instead, the degree of cells synchronized in G2/M is important for high productivity and the gradually decreasing degree of synchronization during the course of a culture might be the explanation behind the cell density dependent decrease in productivity for Sf9 cells. This was further supported by the positive effects on productivity achieved by synchronizing Sf9 cells in G2/M by yeastolate limitation, which counteracted the cell density-dependent drop in productivity and hence a higher volumetric yield was achieved. Addition of 20 % CM to T. ni cultures had a positive effect on productivity. The specific productivity was maintained at a high level longer than for cells in 100 % fresh medium. The product concentration was 34 % higher and the maximum product concentration was obtained 24 hours earlier for the cells with the addition of CM. These results show that the effects of CM on productivity are not the same for the two cell lines and that the mechanism regulating productivity are quite complex.</p>

Biotechnology

Insect cells

BEVS

Spodoptera frugiperda

Sf9

Trichoplusia ni

BTI-Tn-5B1-4

specific productivity

conditioned medium

conditioned medium factors

cell cycle

synchronization

G2/M

Bioteknik

Bioengineering

Bioteknik

Physiological effects of conditioned medium and passage number on Spodoptera frugiperda Sf9 serum free cultures

Svensson, Ingrid

January 2005

<p>The aim of this study was to better understand the role of conditioned medium (CM) in Spodoptera frugiperda Sf9 insect cell proliferation and recombinant protein production using the baculovirus expression system.</p><p>CM was found to stimulate cell proliferation. Addition of CM and 10 kDa CM filtrate to an Sf9 culture decreased the lagphase and the maximum cell density was reached earlier than for cultures in fresh medium. The positive effect of 10 kDa CM filtrate showed that CM contains at least one small growth promoting factor. The effect was not eliminated by trypsin treatment. Addition of CM or 10 kDa CM filtrate to Sf9 cultures was found to have a negative effect on the recombinant protein production. The effect was thought to be indirect and most probably via the impact of CM on cell physiology. CM was also found to contain proteinase activity. The proteinase was identified as Sf9 cathepsin L. A proform with a molecular mass about 49 kDa and two active forms at about 39 and 22 kDa were found. The role of cathepsin L in Sf9 cultures is not yet clear. However, the knowledge of the presence of this proteinase in CM can be of great value for improving product quality and yield. Further, CM was found to have other properties as well: a concentrated fraction of CM exhibited strong antibacterial activity towards Bacillus megaterium and a weaker activity towards Escherichia coli. B. megaterium lysed rapidly after incubation in the CM fraction.</p><p>Repeated subculturing of Sf9 cells provoked a switch in growth kinetics. After 30-45 passages the cells started to proliferate earlier after inoculation and addition of CM had no longer a growth stimulating effect. However, CM still stimulated growth of a culture with low passage (LP) number (up to 45 passages). High passage cells (HP cells, over 100 passages) displayed a shorter lagphase than LP cells and the culture reached the maximum cell density 24-48 h earlier. Cell cycle analysis showed that the Sf9 cells were transiently synchronised in the G2/M phase 10 h after inoculation, before proliferation was initiated. This synchronisation was more pronounced for HP cells than for LP cells, which correlated to a higher recombinant protein production in baculovirus infected HP cells than in LP cells. Synchronisation of cells in G2/M by yeastolate-limitation before infection with baculoviruses suggested that the degree of synchronisation is connected to the cell density dependent decrease in recombinant protein production of Sf9 cultures.</p>

Biotechnology

Spodoptera frugiperda Sf9

insect cell cultures

conditioned medium

cell cycle phase dynamics

proteolytic activity

antibacterial activity

recombinant protein production

Bioteknik

Bioengineering

Bioteknik

Analyse transcriptionnelle des phases précoces de l'infection par le baculovirus AcMNPV et exploitation d'une banque d'ADN complémentaire issue de sa cellule-hôte, Sf9

Landais, Igor

16 December 2002

Le lépidoptère Spodoptera frugiperda est un ravageur important des cultures mais aussi l'organisme source de la lignée cellulaire Sf9, utilisée pour la production de protéines recombinantes dans le système d'expression baculovirus/cellule d'insecte. Dans la première partie de ce travail, nous avons étudié la transcription chez le baculovirus AcMNPV aux temps précoces de l'infection. Nous montrons tout d'abord que les régions homologues (hrs) portées par le génome de ce virus contiennent de nombreux motifs de reconnaissance pour des facteurs de transcription de type AP1/CREB, et que ces sites fixent spécifiquement des protéines de la cellule-hôte, Sf9. Par ailleurs, dans le contexte de l'infection, ces sites sont nécessaires à la transactivation médiée par le facteur viral très précoce IE1 qui se fixe lui aussi sur les hrs. Cette étude montre pour la première fois l'implication de facteurs cellulaires dans ce mécanisme de transactivation virale. La progression de ces travaux a cependant été freinée par le peu de données disponibles sur les gènes exprimés par Sf9. Pour en faciliter l'accès, nous avons donc construit une banque d'ADNc, dont l'exploitation fait l'objet de la deuxième partie de ce mémoire. Son criblage a permis d'obtenir la séquence complète de l'ADN complémentaire du gène hsp90 chez S. frugiperda, et d'en déterminer les principales caractéristiques. Par ailleurs, le séquençage à grande échelle de la banque a conduit à la constitution d'une banque d'ESTs, permettant l'identification de la quasi-totalité des gènes de protéines ribosomales. L'analyse de leur séquence a révélé l'existence de particularités qui semblent restreintes aux insectes et aux lépidoptères, un résultat inattendu compte tenu de la grande conservation de ces gènes entre espèces.

AcMNPV

baculovirus

banque d'ADNc

CRE

CREB

EST

facteur de transcription

transactivation

génomique

hsp90

IE1

lépidoptère

protéine ribosomale

région homologue

Sf9

Spodoptera frugiperda

Age related seroepidemiological survey of measles, mumps, rubella, varicella zoster, herpes simplex type 1 and 2 viruses

Wong, Kiing Aik

January 2015

Age stratified seroepidemiological studies play a crucial role in the design and assessment of vaccination strategies. An existing multiplex bead immunoassay for measles, mumps, rubella and varicella zoster virus antibodies together with a newly developed multiplex bead immunoassay for herpes simplex virus type 1 and type 2 antibodies were used to investigate the age-related seroepidemiology of these viruses in England during 2012.To develop the HSV-1 and HSV-2 antibody assay, attempts were made to produce full length of HSV-1 and HSV-2 glycoprotein G using a baculovirus vector expression system. While HSV-1 gG protein was produced, the proteins were extensively aggregated. Native glycoprotein G molecules undergo partial removal of HSV-1 signal sequence and HSV-1 short membrane anchor sequence during post translational modification. It is possible that such post translational modification is not performed when protein is processed in insect cell culture. Attempts to produce an HSV-2 glycoprotein G were not successful. It is possible that the high GC-content of HSV-2 glycoprotein G led to poor fidelity of copying the PCR amplification sequence. Commercially available truncated HSV-1 gG and HSV-2 gG were therefore used to develop a duplex microbead immunoassay for the simultaneous detection of specific HSV antibodies in human sera. The resultant assays performed with low sensitivity and specificity (HSV-1 of 89% and 66%, respectively and for HSV-2 of 79% and 85%, respectively) compared to the reference HerpeSelect ELISA.The MMRV multiplex bead immunoassay proved rapid, and required minimal sample volume to semi-quantify MMRV specific antibodies. The seroepidemiology of MMR results was compared with previous seroepidemiological studies performed in 1996 in England. The comparison showed an increase in the proportion of individuals who were positive for mumps and measles antibodies in the 2012 survey. The proportion of individuals positive for rubella was essentially unchanged. The increase in the proportion of individuals positive for mumps and measles antibodies in 2012 show the effectiveness of the change in MMR vaccination policy for England from 1996 onward. For VZV, the proportion of individuals who were positive for varicella antibodies between the 1996 and 2012 serological surveys were essentially unchanged. The comparison showed that most young children are susceptible to VZV. At this level of immunity, it can be expected that varicella will continue to produce epidemics of infection in the population, unless varicella vaccination is implemented as a part of routine childhood vaccination.

614.4

Physiological effects of conditioned medium and passage number on Spodoptera frugiperda Sf9 serum free cultures

Svensson, Ingrid

January 2005

The aim of this study was to better understand the role of conditioned medium (CM) in Spodoptera frugiperda Sf9 insect cell proliferation and recombinant protein production using the baculovirus expression system. CM was found to stimulate cell proliferation. Addition of CM and 10 kDa CM filtrate to an Sf9 culture decreased the lagphase and the maximum cell density was reached earlier than for cultures in fresh medium. The positive effect of 10 kDa CM filtrate showed that CM contains at least one small growth promoting factor. The effect was not eliminated by trypsin treatment. Addition of CM or 10 kDa CM filtrate to Sf9 cultures was found to have a negative effect on the recombinant protein production. The effect was thought to be indirect and most probably via the impact of CM on cell physiology. CM was also found to contain proteinase activity. The proteinase was identified as Sf9 cathepsin L. A proform with a molecular mass about 49 kDa and two active forms at about 39 and 22 kDa were found. The role of cathepsin L in Sf9 cultures is not yet clear. However, the knowledge of the presence of this proteinase in CM can be of great value for improving product quality and yield. Further, CM was found to have other properties as well: a concentrated fraction of CM exhibited strong antibacterial activity towards Bacillus megaterium and a weaker activity towards Escherichia coli. B. megaterium lysed rapidly after incubation in the CM fraction. Repeated subculturing of Sf9 cells provoked a switch in growth kinetics. After 30-45 passages the cells started to proliferate earlier after inoculation and addition of CM had no longer a growth stimulating effect. However, CM still stimulated growth of a culture with low passage (LP) number (up to 45 passages). High passage cells (HP cells, over 100 passages) displayed a shorter lagphase than LP cells and the culture reached the maximum cell density 24-48 h earlier. Cell cycle analysis showed that the Sf9 cells were transiently synchronised in the G2/M phase 10 h after inoculation, before proliferation was initiated. This synchronisation was more pronounced for HP cells than for LP cells, which correlated to a higher recombinant protein production in baculovirus infected HP cells than in LP cells. Synchronisation of cells in G2/M by yeastolate-limitation before infection with baculoviruses suggested that the degree of synchronisation is connected to the cell density dependent decrease in recombinant protein production of Sf9 cultures. / QC 20101222

Biotechnology

Spodoptera frugiperda Sf9

insect cell cultures

conditioned medium

cell cycle phase dynamics

proteolytic activity

antibacterial activity

recombinant protein production

Bioteknik

Industrial Biotechnology

Industriell bioteknik

Fonction régulatrice du domaine de projection de MAP2b sur la formation de prolongements cytoplasmiques dans les cellules Sf9

Bélanger, Dave

02 1900

Mémoire numérisé par la Direction des bibliothèques de l'Université de Montréal. / Lors de leur différenciation, les neurones développent deux types de prolongements cytoplasmiques, dendrites et axones. L'élaboration de ces prolongements est médiée par les éléments du cytosquelette, plus particulièrement, les microtubules et les microfilaments d'actine (actine-F). L'expression de la protéine associée aux microtubules-2 (MAP-2) est nécessaire au développement des neurites mineures, les premiers prolongements cytoplasmiques émis par un neurone. Ceux-ci n'ont pas une identité dendritique ou axonale. Par la suite, l'expression de MAP2 est nécessaire au développement et au maintien des dendrites. L'expression de MAP2 est régulée par épissage alternatif au cours de la différenciation neuronale. Il existe quatre isoformes de la protéine MAP2, MAP2a, MAP2b, MAP2c et MAP2d. MAP2b et MAP2c sont les isoformes les mieux caractérisées. Elles peuvent être subdivisées en deux domaines: un domaine de liaison aux microtubules situé en C-terminal et un domaine de projection en N-terminal. Le domaine de liaison aux microtubules est responsable de l'interaction de MAP2 avec les microtubules alors que le rôle du domaine de projection n1est toujours pas clairement défini. MAP2c est exprimée dans les neurones immatures alors que MAP2b est présente dans les neurones immatures et matures. Dans les neurones immatures, ces deux isoformes se retrouvent dans les neurites mineures et elles sont ciblées préférentiellement dans les dendrites au cours de la différenciation neuronale. Le rôle respectif de MAP2b et MAP2c dans l'élaboration de prolongements cytoplasmiques par un neurone demeure inconnu. MAP2b et MAP2c diffèrent par la présence d'une séquence additionnelle de 1372 acides aminés dans le domaine de projection de MAP2b. L'insertion d'une séquence aussi importante dans le domaine de projection de MAP2b indique que ce domaine joue un rôle important. Le but de la présente étude consiste à mieux comprendre le rôle de cette séquence dans la fotmation de prolongements cytoplasmiques. Pour cette analyse fonctionnelle, nous avons produit six formes tronquées de MAP2b qui contiennent des délétions dans le domaine de projection de MAP2b. Ces formes tronquées de MAP2b ont été exprimées dans les cellules ovariennes Spodoptera frugiperda (Sf9). En effet, ce système cellulaire est très intéressant puisque nous avons démontré que l'expression de MAP2b et MAP2c dans ces cellules résulte en la formation de prolongements cytoplasmiques. Cependant, ces deux isoformes de MAP2 induisent des patterns distincts de formation de prolongements cytoplasmiques. 60% des cellules qui expriment MAP2c développent des prolongements alors que 14% des cellules qui expriment MAP2b ont des prolongements. De plus, les cellules qui expriment MAP2c ont la tendance à développer des prolongements multiples alors que celles qui expriment MAP2b présentent un seul prolongement. Nos présents résultats démontrent que le domaine de projection de MAP2b a un effet inhibiteur sur la capacité du domaine de liaison aux microtubules à induire la formation de prolongements cytoplasmiques. En effet, 53% des cellules qui n'expriment que le domaine de liaison aux microtubules ont des prolongements en comparaison à 14% des cellules qui expriment MAP2b. De plus, l'expression de trois formes tronquées de MAP2b qui ont une délétion partielle de la séquence additionnelle de 1372 acides aminés induit un plus grand pourcentage de cellules avec prolongements (27%, 31 % et 41 % ). Toutefois, la séquence commune à MAP2c et MAP2b qui est située à l'extrémité 5' du domaine de projection semble favoriser la formation de plusieurs prolongements puisque sa délétion résulte en un plus faible pourcentage de cellules avec des prolongements multiples. Nos résultats suggèrent donc que l'insertion de la séquence additionnelle de 1372 acides aminés dans le domaine de projection de MAP2b diminue sa capacité à induire la formation de prolongements cytoplasmiques. Étant donné que MAP2b et MAP2c sont capables de se lier à l'actine-F et aux microtubules, nous avons examiné la distribution de ces deux éléments du cytosquelette dans les cellules Sf9 qui expriment les différentes formes tronquées de MAP2b. Toutes les formes tronquées de MAP2b induisent la formation de faisceaux de microtubules à l'exception des formes tronquées qui correspondent aux domaines de projection de MAP2c et de MAP2b. Dans les cellules qui présentent des prolongements, on note une réorganisation de l'actine-F. Dans les cellules qui expriment la forme mutante correspondant au domaine de projection de MAP2b, l'actine-F est distribuée sous forme d'un anneau sous la membrane plasmique. De plus, le domaine de projection a une distribution similaire. Ceci suggère que le domaine de projection de MAP2b interagit avec l'actine-F. Donc la séquence additionnelle de 13 72 acides aminés pourrait contenir un domaine de liaison à l'actine. En conclusion, nos résultats indiquent que MAP2b aurait une moins grande capacité que MAP2c à promouvoir la formation de neurites mais elle pourrait contribuer à leur stabilisation au cours de la différenciation neuronale par le fait qu'elle contient des domaines additionnels de liaison à l'actine.

Différenciation neuronale

Neurites

Microtubules

Microfilaments d'actine (actine-F)

Isoformes MAP2a, MAP2b, MAP2c, MAP2d

Cellules Sf9