O TRANSPOSON piggyBac: QUANTIFICANDO SUA MOBILIZAÇÃO / A new way to quantify transposon mobilization using piggyBac as model

Kaminski, Valéria de Lima

05 May 2015

Conselho Nacional de Desenvolvimento Científico e Tecnológico / In this work we presented the idea to perform excision assays using the piggyBac transposable element as enzyme supplier and the inverted terminal sequences of the element, both necessary for mobilization of a transposable element. Drosophila S2 cells were electroporated to perform insertion of two different plasmids in the cytoplasm of cells, a plasmid carrying the terminal inverted repeats of piggyBac element flanking a GFP gene and other with the transposase coding sequence enzyme which recognizes the terminal inverted repeats, excise of the region where the element is and insert it into another locus. This is a vector-helper system, in which a fragment is excised from a plasmid with the help of the transposase located in the other. Conventional PCR was used to verify excision events showing a 200bp amplification region where the fragment was excised and a region 3kb amplification reagion at times when the fragment was full, ie, it has not mobilized. The qPCR technique was used to quantify the excision of this fragment, carrying out comparisons of the amount of plasmid DNA recovered from the S2 cells after the end of experiment with serial dilutions of the original plasmids carrying the ITRs, which was used as standard. The results showed that the technique involving electroporation and qPCR is feasible and can be used to quantify mobilization of transposable elements. Paralleling with existing tools for this type of quantification, qPCR shows up as a very sensitive technique of detection mobilization, as well as a low cost technique budget. / Neste trabalho apresentamos a ideia de realizar ensaios de excisão utilizando o elemento transponível piggyBac como fornecedor da enzima e das sequências terminais invertidas do elemento, ambos necessários para mobilização. Células S2 de Drosophila melanogaster foram eletroporadas para que houvesse inserção de dois diferentes plasmídeos no citoplasma das células, um plasmídeo portando as repetições terminais invertidas do elemento piggyBac flanqueando um gene GFP e o outro com a sequência codificadora da enzima transposase, a qual reconhece as repetições terminais invertidas e excisa o elemento da região onde está inserido, num sistema vector-helper, em que um fragmento é excisado de um plasmídeo com ajuda da transposase localizada no outro. PCR convencional foi usado para verificar os eventos de excisão, mostrando uma região de amplificação de 200pb nos casos de excisão do fragmento e uma região amplicada de 3kb, nas ocasiões em que o fragmento ficou inteiro, ou seja, não foi mobilizado. A qPCR foi utilizada para quantificar a excisão desse fragmento, realizando comparações da quantidade de DNA plasmidial recuperado das células S2 após o término do experimento com diluições em série do plasmídeo com as ITRs, que foi utilizado como standard. Os resultados mostraram que a técnica envolvendo eletroporação e qPCR é exequível e pode ser utilizada para quantificar mobilização de elementos transponíveis. Fazendo um paralelo com as ferramentas já existentes para esse tipo de quantificação, qPCR mostra-se como uma técnica bastante sensível de detecção de mobilização, bem como uma técnica de baixo custo orçamentário.

Células S2

PiggyBac

Excisão

Eletroporação

QPCR

S2 cell lineage

PiggyBac

Excision

Electroporation

QPCR

CNPQ::CIENCIAS BIOLOGICAS

Phenotypic Variations In Animal Morphogenesis : Sea Urchin Twins And Cloned Rabbits / Variations phénotypiques de la morphogénèse animale : jumeaux d'oursins et lapins clonés

Fabrèges, Dimitri

11 January 2016

La variabilité est une propriété intrinsèque aux systèmes biologiques, essentielle pour l'évolution et l'embryogénèse. Souvent considérée comme du bruit, ce n'est que récemment que l'aléatoire des processus biologiques a commencé à être systématiquement étudié. Cette thèse pose les questions suivantes : qu'est-ce qu'un développement normal ? Quel est l'étendue et le rôle de la variabilité dans la robustesse et la résilience du développement embryonnaire ?Ces questions sont posées pour le lapin (Oryctolagus cuniculus) et l'oursin (Paracentrotus lividus et Sphaerechinus granularis).Nous nous sommes aussi intéressé à la quantification du déterminisme de la variabilité embryonnaire à l'aide d'oursins jumeaux et de lapins clonés.La mesure des comportements cellulaires est effectuée sur des lignages cellulaires obtenus à partir d'imagerie 3D+temps. Nous montrons que les oursins jumeaux peuvent se développer selon trois phénotypes différents, jamais observés chez le normal, avant de converger vers une blastula d'apparence normale. De plus, les comparaisons entre et au sein des pairs de jumeaux montrent que le phénotype et la survie ne dépend que de l'histoire individuelle des embryos.Nos mesures quantitatives des pairs de jumeaux amènent des questions ouvrant de nouveaux horizons de recherche : les jumeaux sont-ils robustes ou résilient ?Le développement pré-implantatoire des lapins a été étudié sur cinq embryons numériques (trois sauvages et deux clones), du stade 32-cellules à l'éclosion.Nous montrons que les divisions asymétriques internes et externes régulent la variation du nombre de cellules internes ainsi que la taille de la masse cellulaire.De plus, la variation du nombre de cellules internes est plus grande que pour les cellules externes, ce qui semble directement lié au taux de morts cellulaires.Notre hypothèse est que le potentiel de bon développement des clones est assuré par une grande plasticité épigénétique des cellules donneuses.Ce travail espère définir des méthodes et des concepts fondateurs pour une exploration quantitative et une modélisation multi-échelle de la morphogénèse animale. / Variability is an intrinsic characteristic of biological systems, essential for evolution and embryogenesis.Considered as noise for centuries, it is only recently that the stochasticity of biological processes has began to be systematically explored.The present thesis addresses the following questions: What is a normal development?What is the extent and role of variability in developmental robustness and resilience?We tackle these issues in rabbit (Oryctolagus cuniculus) and sea urchin (Paracentrotus lividus and Sphaerechinus granularis).We also aimed to quantify determinism and stochasticity of developmental variability by means of sea urchin twins and cloned rabbits.Variations in cell behaviors were investigated through reconstruction of cell lineage from 3D+time imaging.We showed that sea urchin twins can follow three different developmental paths never observed in normal embryo, before converging to normal looking blastula.Moreover, comparisons between and within pairs of twins revealed that phenotype and survival depend on individual history alone.Our quantitative observation of twin pairs raises question opening a future line of research: are twins robust or resilient?Rabbit preimplantation development was explored with five digital specimens (three wild-types and two clones) from the 32-cell stage to hatching.We showed that inner and outer asymmetric divisions regulate the variation of inner cell number and may control inner cell mass size.In addition, the variation of inner cell number in clones is higher than outer cells which seems to be directly correlated to their cell death ratio.Our current hypothesis is that the potential to lead to viable clones requires plasticity of donor's epigenetic state.This work is expected to ground concepts and methods for a quantitative exploration and further multilevel modeling of morphogenetic processes.

Variabilité

Quantification

Morphogénèse

Lignage cellulaire

Oursins

Lapins

Variability

Quantification

Morphogenesis

Cell lineage

Sea urchins

Rabbits

Genomic instability may be a signal of human embryonic stem cell differentiation

Esteban-Perez, Clara Ines

30 April 2011

Embryonic stem (ES) cells have the ability to maintain pluripotency and self-renewal during in vitro maintenance, which is a key to their clinical applications. ES cells are a model in developmental biology studies due to their potential to differentiate in vitro. Understanding critical pathways of pluripotency, self-renewal, and differentiation during early embryonic development is important for the evaluation of the therapeutic potential of ES cells because of their ability for tumor transformation due to genetic and epigenetic instability acquired during in vitro culture maintenance. Single tandem repeats are sequences of DNA that have been implicated in the deregulation of gene expression in different human conditions. Understanding the origin of repetitive sequence instability and functions in the genome allow characterization of early genomic instability signals in ES cell pluripotency, differentiation, and tumor transformation pathways. The hypothesis of this study was that genetic stability, in repetitive sequences, located near embryonic developmental genes is responsible for pluripotency, self-renewal, differentiation, and chromatin assembly and could be a signal for adaptation, differentiation, or transformation of ES cells in vitro. Our result showed instability in specific repetitive sequences which increased during ES cell passages and embryoid body differentiation in vitro. ES cells displayed significant mean frequencies of genomic instability in repetitive regions that lead to ES cells pluripotency, self-renewal maintenance, or cell lineage specialization. The present study reports potentially biomarkers for identifying accumulation of genomic instability in specific genes that may contributes to adaptation of ES cells and could be the switch that initiates early ES cell lineage commitment in vitro. Determining genetic and epigenetic modifications, including single tandem repeat instability, gene expression changes, and chromatin modifications, is essential for elucidating possible molecular mechanisms of genomic instability and determining novel molecular characterization for diagnostic purposes to ensure ES cell stability and integrity that could potentially lead to use of ES cell derivatives that could then be a safe source needed for regenerative medicine applications

genomic instability

cell lineage commitment

cell differentiation

pluripotency

Embryonic stem cell

repetitive sequences

tumor transformation

Parameter Analysis in Models of Yeast Cell Polarization and Stem Cell Lineage

Renardy, Marissa

10 August 2018

No description available.

Mathematics

mathematical biology

computational biology

parameter estimation

sensitivity analysis

cell polarization

cell lineage

Mecanismos envolvidos na morte e sobrevivência de linfócitos expostos ao ácido palmítico. / Mechanisms involved in death and survival of lymphocytes exposed to palmitic acid.

Takahashi, Hilton Kenji

31 August 2010

Ácidos graxos podem atuar na apoptose ativando e/ou desativando sinais que regulam este processo. Células Jurkat (linhagem de linfócitos-T) foram tratadas com ácido palmítico (PA) (50, 100 e 150µM) e avaliada a ativação de vias de morte e de sobrevivência. O tratamento com PA induziu apoptose pela ativação da via intrínseca de maneira dose-dependente. A exposição destas células ao PA elevou a expressão do receptor de insulina e de GLUT-4, obtendo-se correlação positiva com a apoptose. O mesmo foi observado em linfócitos humanos expostos ao PA e de linfócitos de ratos em jejum. O tratamento das células Jurkat com insulina após exposição ao PA promoveu a ativação da via de sinalização insulínica. O PA aumentou a captação de glicose, mas observou-se diminuição de sua oxidação e o acúmulo de lípides. Assim, a via de sinalização da insulina e o metabolismo de glicose não oxidativo são estimulados como parte de uma coordenada resposta de sobrevivência de linfócitos expostos ao PA em baixas concentrações, mas em altas concentrações ocorre apoptose. / Fatty acids affect apoptosis pathway activating or deactivating signals that regulate this process. Jurkat cells (T-lymphocyte lineage) were treated with sub-lethal concentrations of palmitic acid (PA) (50, 100 e 150µM) and the cell death and survival signaling pathways were investigated. PA induced apoptosis in a dose dependent manner activating the intrinsic pathway. Jurkat cells exposed to PA showed increased insulin receptor and GLUT-4 expression and a positive correlation with apoptosis was obtained. Similar effect was observed in human lymphocytes exposed to PA and lymphocytes from fasted rats. Insulin treatment of Jurkat cells after PA exposure promoted the activation of the insulin signaling pathway. Glucose uptake was increased in the presence of PA, however, its oxidation was diminished and ncreased of lipids accumulation. Therefore, insulin signaling and non oxidative glucose metabolism are stimulated as a part of a coordinated response to survival of lymphocytes exposed to low concentration of PA but in high concentration it induces apoptosis.

Ácidos graxos

Apoptose

Apoptosis

Cell lineage

Cell metabolism

Fatty acids

Insulin

Insulina

Linfócitos

Linhagem celular

Lymphocytes

Metabolismo celular

Mecanismos envolvidos na morte e sobrevivência de linfócitos expostos ao ácido palmítico. / Mechanisms involved in death and survival of lymphocytes exposed to palmitic acid.

Hilton Kenji Takahashi

31 August 2010

Ácidos graxos podem atuar na apoptose ativando e/ou desativando sinais que regulam este processo. Células Jurkat (linhagem de linfócitos-T) foram tratadas com ácido palmítico (PA) (50, 100 e 150µM) e avaliada a ativação de vias de morte e de sobrevivência. O tratamento com PA induziu apoptose pela ativação da via intrínseca de maneira dose-dependente. A exposição destas células ao PA elevou a expressão do receptor de insulina e de GLUT-4, obtendo-se correlação positiva com a apoptose. O mesmo foi observado em linfócitos humanos expostos ao PA e de linfócitos de ratos em jejum. O tratamento das células Jurkat com insulina após exposição ao PA promoveu a ativação da via de sinalização insulínica. O PA aumentou a captação de glicose, mas observou-se diminuição de sua oxidação e o acúmulo de lípides. Assim, a via de sinalização da insulina e o metabolismo de glicose não oxidativo são estimulados como parte de uma coordenada resposta de sobrevivência de linfócitos expostos ao PA em baixas concentrações, mas em altas concentrações ocorre apoptose. / Fatty acids affect apoptosis pathway activating or deactivating signals that regulate this process. Jurkat cells (T-lymphocyte lineage) were treated with sub-lethal concentrations of palmitic acid (PA) (50, 100 e 150µM) and the cell death and survival signaling pathways were investigated. PA induced apoptosis in a dose dependent manner activating the intrinsic pathway. Jurkat cells exposed to PA showed increased insulin receptor and GLUT-4 expression and a positive correlation with apoptosis was obtained. Similar effect was observed in human lymphocytes exposed to PA and lymphocytes from fasted rats. Insulin treatment of Jurkat cells after PA exposure promoted the activation of the insulin signaling pathway. Glucose uptake was increased in the presence of PA, however, its oxidation was diminished and ncreased of lipids accumulation. Therefore, insulin signaling and non oxidative glucose metabolism are stimulated as a part of a coordinated response to survival of lymphocytes exposed to low concentration of PA but in high concentration it induces apoptosis.

Ácidos graxos

Apoptose

Insulina

Linfócitos

Linhagem celular

Metabolismo celular

Apoptosis

Cell lineage

Cell metabolism

Fatty acids

Insulin

Lymphocytes

The effect of phosphate deficiency on BMP-2 treated C3H10T1/2 mesenchymal stem cells

Bui, Matthew

03 July 2018

There are approximately 600,000 cases of delayed or aberrant fracture healing in people each year, with a small subset of these fractures experiencing disunion. Dietary phosphate deficiency has been shown to impair oxidative phosphorylation and decrease BMP-2 mediated chondrogenic differentiation during fracture healing. Prior studies using pre-committed chondro-progenitor ATDC5 cell line grown in phosphate deficient media showed that energy consumption was linked to protein production and collagen hydroxylation but inversely related to matrix mineralization. The goal of this study was to further define the relationship between energy consumption and BMP-2 mediated stem cell chondrogenic differentiation and further examine how dietary phosphate, and promotion of collagen hydroxylation via ascorbate availability effected these processes. C3H10T1/2 murine cells, a multi-potential cell line, were expanded in pre-differentiation growth medium (DMEM with 10% FBS and 1% Pen/Strep). Once cells reached 60% confluence (day 0), they were grown in differentiating media (α-MEM with 5% FBS and 1X insulin-transferrin-selenium) containing either 100% (1mM) or 25% (0.25mM) inorganic phosphate (Pi), ± 200ng/mL BMP-2(BMP), and ±0.2 mM L-ascorbic acid (AA). In total, there were 8 groups with varying combinations of these three substances. Intracellular lipid, total DNA, protein, and hydroxyproline (HP) content were examined. Chondrocyte gene expression (Col2a1, Acan, ColXa1) and adipocyte gene expression (Pparg, Plin1, Ucp1) were measured to check for cell lineage commitment and specific differentiation of the C3H10T1/2. All measurements were acquired at day 8. The +BMP differentiation media groups contained significantly less DNA content and more protein content than the –BMP differentiation media groups (both p<0.0001). There was also a significant interaction between phosphate and ascorbic acid treatment (p=0.0296), with 25% Pi +AA groups producing significantly more protein than 100% Pi +AA groups. Hydroxyproline production was not different in 100% Pi or 25% Pi conditions (p=0.2951). AA presence in culture media led to greater HP production than culture media lacking AA (p=0.0035) There was a trend of an interaction between phosphate content and AA availability (p=0.0744). 100% Pi ±AA groups produced significantly different amounts of HP while 25% Pi ±AA groups did not produce significantly different amount of HP. Col2a1, Acan, and ColXa1 expression were all increased in +BMP groups. Ascorbic acid treatment groups expressed significantly more Col2a1and Acan than –AA groups. 100% Pi media led to greater Acan expression over 25% Pi groups (p=0.0009), whereas 25% Pi media trended to lead to greater ColXa1 expression over 100% Pi groups (p=0.0734). Pparg and Plin1 expression were increased in the 25% Pi condition. There were no significant differences in expression of Ucp1. C3H10T1/2 cells were significantly affected by phosphate concentration, BMP-2 treatment, and ascorbic acid supplementation. Phosphate deficiency hindered maturation of early chondrocytes into proliferating chondrocytes while also promoting MSC differentiation into the adipocyte cell lineage. Hypertrophic chondrocyte expression was decreased in phosphate deficient media, which may coincide with increased protein production observed in low phosphate conditions. BMP-2 promoted chondrogenesis which resulted in increased protein production. Whereas, lack of ascorbic acid in cell culture media led to decreased hydroxyproline production.

Medicine

Bone development

Bone morphogenetic protein 2

Cell differentiation

Cell lineage commitment

Fracture healing

Mesenchymal stem cell

Mechanisms Regulating Early Mesendodermal Differentiation of Human Embryonic Stem Cells: A Dissertation

VanOudenhove, Jennifer J.

02 June 2016

Key regulatory events take place at very early stages of human embryonic stem cell (hESC) differentiation to accommodate their ability to differentiate into different lineages; this work examines two separate regulatory events. To investigate precise mechanisms that link alterations in the cell cycle and early differentiation, we examined the initial stages of mesendodermal lineage commitment and observed a cell cycle pause that occurred concurrently with an increase in genes that regulate the G2/M transition, including WEE1. Inhibition of WEE1 prevented the G2 pause. Directed differentiation of hESCs revealed that cells paused during commitment to the endo- and mesodermal, but not ectodermal, lineages. Functionally, WEE1 inhibition during meso- and endodermal differentiation selectively decreased expression of definitive endodermal markers SOX17 and FOXA2. These findings reveal a novel G2 cell cycle pause required for endodermal differentiation. A role for phenotypic transcription factors in very early differentiation is unknown. From a screen of candidate factors during early mesendodermal differentiation, we found that RUNX1 is selectively and transiently up-regulated. Transcriptome and functional analyses upon RUNX1 depletion established a role for RUNX1 in promoting cell motility. In parallel, we discovered a loss of repression for several epithelial genes, indicating that RUNX1 knockdown impaired an epithelial to mesenchymal transition during differentiation. Cell biological and biochemical approaches revealed that RUNX1 depletion compromised TGFβ2 signaling. Both the decrease in motility and deregulated epithelial marker expression upon RUNX1 depletion were rescued by reintroduction of TGFβ2, but not TGFβ1. These findings identify novel roles for RUNX1-TGFβ2 signaling in mesendodermal lineage commitment.

Cell Differentiation

Human Embryonic Stem Cells

Cell Cycle

Cell Lineage

Dissertations, UMMS

Cell Biology

Cellular and Molecular Physiology

The embryonic development of Elminius modestus Darwin, 1854

Ponomarenko, Ekaterina

04 August 2014

Die vorliegende Arbeit behandelt die Embryonalentwicklung des Rankenfußkrebses Elminius modestus (Thecostraca: Cirripedia). Der Entwicklungsprozess wurde mithilfe unterschiedlicher Methoden wie 4D Mikroskopie, in vivo Einzelzellmarkierungen, Fluoreszenzhistochemie und konfokaler Laserscanningmikroskopie in Verbindung mit 3D Rekonstruktionen untersucht. Die Furchung von E. modestus ist total, inequal in Bezug auf die Dotterzelle und asynchron mit einem anterior-posterioren Gradienten. Der gesamte Prozess folgt einem strengen Teilungsmuster mit nur sehr geringer Variabilität. Eine davon stellt das Auftreten spiegelbildlicher Embryonen ab dem 4-Zell. Die Keimblattdifferenzierung wurde vor allem mittels in vivo Zellmarkierungen untersucht. Die Trennung der endodermalen und endomesodemalen Keimblätter erfolgt nach der vierten Furchungsteilung, die Trennung des Ectomesoderm nach der sechsten Teilung. Die Urkeimzellen sind aller Wahrscheinlichkeit nach ein Produkt der siebten Furchungsteilung der Dotterzellen (3Da und 3Dp). Im Zuge der Untersuchung konnte die Zelllinie jedes Keimblattes rekonstruiert werden, die Zellschicksale der Abkömmlinge der Quadranten wurde bis zum 16-Zell Stadium beschrieben. Das Ectoderm entspringt allen vier Quadranten, ebenso das Ectomesoderm (die letzten identifizierten Mesectoblasten sind 3A, 3B, 3C, 1drp und 1dlp). Endoderm und Endomesoderm entwickeln sich aus einzelnen Vorläuferzellen im 16-Zell Stadium (2D bzw. 2d). Das Auftreten nur eines einzelnen Endoblasten stellt eine mögliche Apomorphie aller Ecdysozoa dar. Das Vorhandensein eines einzelnen Mesendoblasten wird als mögliches Merkmal des Grundmusters aller Protostomia in Betracht gezogen. / The present work is devoted to the embryonic development of the thoracican barnacle Elminius modestus (Thecostraca: Cirripedia). The developmental process was investigated by means of different techniques like 4D microscopy, in vivo labelling, fluorescent histochemistry, and confocal laser scanning microscopy combined with 3D reconstructions. The cleavage of E. modestus is total, unequal with regards to the yolky cell, and asynchronous with an anterior-posterior gradient. The entire process appears to follow a strict pattern of divisions with very little variability, one of which includes the occurrence of mirror image embryos from the 4-cell stage on. The germ layer differentiation was mainly studied by means of in vivo labelling. The segregation of the endodermal and the endomesodemal germ layers are shown to happen after the fourth division, whereas the ectomesoderm segregates after the sixth division. The primordial germ cells are suggested to be a product of the seventh cleavage division of the yolky cells (3Da and 3Dp). During the research the cell lineage of each germ layer was established, the fates of the quadrant descendants are described up to the 16-cell stage. The ectoderm originates from four quadrants, as does the ectomesoderm (the last identified mesectoblasts are 3A, 3B, 3C, 1drp, and 1dlp). The endoderm and the endomesoderm develop from single precursors at the 16-cell stage (2D and 2d, respectively). The presence of only a single endoblastic cell, might represent an apomorphy for the entire group of Ecdysozoa. A singular mesendoblast is suggested to be a possible feature in the developmental ground pattern of all Protostomia.

Rankenfußkrebse

Krebstiere

Zelllinie

Spiralfurchung

Blastoporus

Endoderm

Ektomesoderm

Endomesoderm

cirripedes

crustaceans

cell lineage

spiral cleavage

blastopore

endoderm

ectomesoderm

endomesoderm

570 Biowissenschaften, Biologie

32 Biologie

WQ 2350

ddc:570

Der postnaupliale Keimstreif von Porcellio scaber und Orchestia cavimana (Crustacea, Peracarida)

Hejnol, Andreas

20 March 2002

Malkostrake Krebse zeigen im postnauplialen Keimstreif ein invariantes Zellteilungsmuster und eine Zelllinie. Embryonen eines Isopoden (Porcellio scaber) und eines Amphipoden (Orchestia cavimana) wurden bezüglich ihrer Zelllinie vergleichend Untersucht. Mittels immunhistochemischer Färbungen wurde das Expressionsmuster der Gene engrailed und Distal-less in Hinblick auf die Zelllinie und die Morphogenese der Segmente und der Beinentwicklung analysiert. Die Zelllinie wurde bei Porcellio scaber mit der Methode der 4D-Mikroskopie untersucht. Mit Zellablationsexperimenten wurden Abhängigkeiten der Zellen untereinander aufgezeigt. Die Ergebnisse dieser Untersuchungen zeigen: I. Die Genexpression von Distal-less und engrailed wird unabhängig von der Zelllinie reguliert. II. Die Bildung der konvergenten einästigen Beine im Thoraxbereich beider Krebse erfolgt durch unterschiedliche Regulation des Gens Distal-less - bei Orchestia cavimana wird die Expression des Gens in den lateralen Zellen abgeschaltet, während diese Zellen bei Porcellio scaber erst gar nicht Distal-less exprimieren. III. Die Anwendung des Systems der 4D-Mikroskopie zeigte unter anderem, dass in den vorderen Reihen nichtektoteloblastischen Ursprungs bei Porcellio scaber die Zelllinie variabel ist und eine Zellsortierung und Zellimmigration stattfindet. IV. Die Ähnlichkeit der Bildung dieser Reihen bei Porcellio scaber mit der der Tanaidaceen lässt auf ein Schwestergruppenverhältnis der Taxa Isopoda und Tanaidacea schliessen. Die Dissertation enthält fünf Videoaufnahmen als separate AVI-Dateien. / Malacostracan crustaceans show in their postnaupliar germ-band an invariant cleavage pattern and a cell-lineage. A comparative analysis of this cell-lineage in an Isopod (Porcellio scaber) and an amphipod (Orchestia cavimana) was done in this thesis. Immunohistochemical stainings of the gene products Distal-less and Engrailed were used, to show the relation of these genes to the morphogenesis of segments and legs. Further, the cell-lineage of Porcellio scaber was analyzed with a 4D-microscope system. Cell-ablation experiments were used to show regulational networks in the development of the germ-band. The results of this work show: I. The regulation of the genes Distal-less and engrailed is independent of the cell-lineage. II. The morphogenesis of the convergent monoramous limbs in the thorax is reflected by different expression patterns of the gene Distal-less - in Orchestia cavimana the expression of Distal-less is switched off in the lateral cells, in Porcellio scaber these cells do not start the Distal-less expression. III. The 4D-microscopy analysis show, that the cell-lineage in the cellrows wich have a non-ectoteloblastic origin is not invariant. In these rows of cells show cell sorting. IV. The formation of these rows in the isopod Porcellio scaber shows similarity to the formation in tanaidaceans. A sister group relationship of Tanaidacea and Isopoda is strongly supported. This dissertation contains five video recordings as separate AVI files.

Crustacea

Zelllinie

Distal-less

engrailed

Zell-Ablation

4D-Mikroskopie

cell-lineage

crustacean

Distal-less

engrailed

cell-ablation

4D-microscopy

570 Biowissenschaften, Biologie

32 Biologie

WX 6423

ddc:570