Molecular-cytogenetic analysis of repetitive sequences in genomes of Beta species and hybrids

Dechyeva, Daryna

07 July 2006

The elucidation of the composition and organization of genomes of higher plants is a fundamental problem of modern molecular biology. The genus Beta containing 14 species assigned to the sections Beta, Corollinae, Nanae and Procumbentes provides a suitable system for the comparative study of the nuclear genomes. Sugar beet Beta vulgaris has a genome size of 758 Mbp DNA with estimated 63 % repetitive sequences and the number of chromosomes n=9. The wild beet Beta procumbens is an important natural pool of resistance against pests and tolerance to unfavorable growth conditions. The subject of this research was the isolation and description of new repetitive DNA families from genomes of this Beta species. This work presents the molecular investigation and cytogenetic characterization by high-resolution multicolor fluorescent in situ hybridization (FISH) of the satellite and dispersed repetitive sequences in wild and cultivated beet species and in their hybrids. New repetitive sequences were isolated from the B. procumbens genome. The AluI restriction satellite repeats pAp11 are 229-246 bp long and form subfamilies. The satellite is amplified in the section Procumbentes, but also found in distantly related section Beta. Thus, pAp11 is probably an ancient component of Beta genomes. It could be the ancestor of the satellite subfamily pEV4 in B. vulgaris based on sequence analysis, Southern hybridization and comparative FISH. pAp11 was found at centromeric and a few intercalary sites in B. procumbens and formed intercalary blocks on B. vulgaris chromosomes where it co-localized with pEV4. These remarkable differences in the chromosomal position of pAp11 between Procumbentes and Beta species indicate that both satellites were likely involved in the expansion or rearrangement of the intercalary heterochromatin of B. vulgaris. Other two sequence families characterized on molecular, genomic and chromosomal levels are the non-homologous repeats pAp4 and pAp22, 1354 and 582 bp long. They have a dispersed organization in the genome and are widely scattered along B. procumbens chromosomes. pAp4 and pAp22 are specific for the section Procumbentes and can be used as DNA probes to discriminate parental genomes in interspecific hybrids. High-resolution FISH on meiotic chromosomes showed that the both sequences mostly co-localize. The PCR analysis of their flanking regions revealed that pAp22 is a part of a Long Terminal Repeat (LTR) of an Athila-like env-class retrotransposon. This is the first indication that the retrovirus-like DNA elements exist in Beta. An ancient family of subtelomeric satellite DNA pAv34 was isolated from all four sections of the genus Beta and from spinach, a related Chenopodiaceae. Five clones were analyzed from each of the five species. The genomic organization and species distribution of the satellites were studied by sequencing and Southern hybridization. The repeating units in all families are 344-362 bp long and share 46.2-98.8 % similarity. Each monomer consists of two subunits SU1 and SU2 of 165-184 bp. The maximum likelihood and neighbor joining analyses of the 25 subtelomeric satellite monomers and their subunits indicated, that the duplication leading to the emergence of the 360 bp satellite should have occurred early in the phylogeny. The two directions of diversification are the clustering of satellites in two groups of subunits SU1 and SU2 and the arrangement of satellite repeats in section-specific groups. The comparative chromosomal localization of the telomeric repeat, pAv34 and rDNA was investigated by multicolor FISH. B. vulgaris chromosome termini showed unique physical organization of telomeric repeat and the subtelomeric satellite, as studied by high-resolution FISH on extended DNA fibers. The estimated length of the telomeric array was 0.55 - 62.65 kb, the length of pAv34 was 5.0-125.25 kb, the spacer between these sequences spanned 1.0-16.60 kb. Eight various classes of repeats were used to characterize the minichromosomes of the sugar beet fragment addition lines PRO1 and PAT2 by comparative multi-color FISH. The study allowed to propose a schematic pattern of repetitive DNA organization on the PRO1 and PAT2 minichromosomes. PRO1 has an acrocentric minichromosome, while PAT2 possesses a metacentric or submetacentric chromosome fragment. The functional integrity of the fragment addition line centromeres was confirmed by an immunostaining localization of the proteins specific to the active kinetochore. The serine 10-phosphorylated histone H3 was detected in pericentromeric regions of the PRO1 chromosomes. The microtubuli attachment sites were visualized as parts of kinetochore complexes.

info:eu-repo/classification/ddc/570

ddc:570

Évaluation de la fréquence des micronoyaux et du potentiel clastogène et/ou aneugène du benzo-a-pyrène suite à une exposition in vitro des lymphocytes humains

Pham, Thi Cam Van

04 1900

No description available.

Génotoxicité

Aberrations chromosomiques

Sonde pancentromérique

Centromères

Courbe dose-réponse non linéaire

Différence interindividuelle

Différence intersexe

Progression

Cancer

Genotoxicity

Chromosome aberrations

Pancentromeric probe

Centromeres

Non-linear dose-response curve

Interindividual differences

Sex differences

Progression

Cancer

Rôles des facteurs de transcriptions SIM1, OTP et POU3F2 dans le développement de l'hypothalamus antérieur

St-Onge, Sandrine

04 1900

Les facteurs de transcription SIM1, OTP, POU3F2 et ARNT2 interagissent ensemble en orchestrant le développement complexe de l’hypothalamus, une région du cerveau contenant plusieurs petites populations circonscrites de neurones, dont le noyau paraventriculaire (PVN). Ce noyau est un important centre intégrateur et l’haploinsuffisance du facteur de transcription Sim1, essentiel au développement du PVN, mène à l’hyperphagie autant chez la souris que l’homme. Différentes souris ont été générées par génie génétique afin de nous aider à trouver d’autres gènes essentiels qui participent à cette cascade transcriptionnelle. Premièrement, la partie antérieure de l’hypothalamus a été récoltée chez des embryons (E12.5) de souris qui surexprimaient le gène Pou3f2 sous le promoteur de Otp7. L’analyse transcriptionnelle de cette partie a été comparée avec les embryons (E12.5) wt de la même portée, de sorte qu’il a été possible de constater que différents gènes ont été régulés à la hausse et d’autres à la baisse. Les gènes en question ont été choisis selon leur pertinence au développement de la région d’intérêt, l’hypothalamus, et de trois autres critères : un accroissement de plus de 1.5, une expression minimale dans l’embryon d’au moins 1000 lectures et le rang le plus haut. Cette méthode discriminatoire a permis d’identifier les gènes les plus affectés dont Lgi2, Fezf2, Sema3c, Six6, Sox14, Lmo4, Nwd2 et Nkx2.1. Les gènes régulés à la baisse étaient Six6, Sox14 et Nkx2.1, tandis que tous les autres étaient à la hausse. Afin de confirmer les résultats obtenus, une validation par hybridation in situ a été utilisée sur des tranches d’hypothalamus d’embryons E12.5. Nous avons pu confirmer la surexpression des marqueurs Lgi2, Fezf2, Sema3c, Lmo4 et de Pou3f2 dans le domaine du PVN. La diminution de l’expression des marqueurs Sox14 et Nkx2.1 a pu être détectée dans el domaine basal de l’hypothalamus, ce qui suggère que l’effet d’une surexpression de Pou3f2 dans le domaine du PVN ait un effet cellulaire non autonome. La diminution de l’expression de Six6 dans le domaine basal n’a pas pu être confirmer de façon reproductible. Deuxièmement, il semblerait qu’il y ait une redondance de rôle entre les facteurs de transcription Otp et Sim1, tous les deux agissant en amont de Pou3f2. Afin de comparer leur impact dans le programme transcriptionnel, la technologie CrisPR-cas9 a été utilisée pour faire un KO du 2e exon d’Otp. Nous avons pu confirmer notre modèle de mutation en le comparant aux autres mutants de la littérature par une réduction de l’expression d’OT, d’OTP, d’AVP et de TRH. Troisièmement, les souris hétérozygotes pour Otp et Sim1 seront croisées, de sorte d’obtenir quatre génotypes : wt, Otp+/-, Sim1+/tlz+ et Otp+/-Sim1+/tlz+. Puisqu’une redondance des rôles de Sim1 et Otp est soupçonnée, le phénotype du double mutant devrait présenter une obésité par hyperphagie plus importante que celle des souris hétérozygotes pour le gène Sim1 ou Otp. Les souris sont pesées à partir de la 5e semaine de vie jusqu’à l’âge de 6 mois à une fréquence d’une fois par semaine. L’apport calorique est également mesuré une fois par semaine sur période de 24h. La double mutation (Otp+/-Sim1+/tlz+) chez les souris mâles causait un phénotype d’obésité plus important que la singularité des mutations, mais ce n’était pas le cas chez les souris femelles. Les souris portant la mutation d’Otp étaient tout de même plus obèses que les souris sauvages pour les deux sexes. Plus de souris seront nécessaire pour déterminer si un apport calorique sans changement au niveau des dépenses énergétiques est la cause de ce gain pondéral. / The transcription factors SIM1, OTP and POU3F2 interact together to orchestrate the complex development of the hypothalamus, a region of the brain containing several small, circumscribed populations of neurons, including the paraventricular nucleus (PVN). This nucleus is an important integrating center, and the haploinsufficiency of the transcription factor Sim1, essential for the development of PVN, leads to overeating in both mice and humans. Different mice have been genetically engineered to help us find other essential genes that participate in this transcriptional cascade. Firstly, the anterior part of the hypothalamus was collected from mice embryos (E12.5) which overexpressed the Pou3f2 gene under the OTP7 promotor. The transcriptional analysis was compared to wt embryos from the same litter to see the different upregulated and downregulated genes. These genes were chosen according to their relevance to the development of the anterior hypothalamus. Three criteria were used to discriminate genes from one another: 1) an increase of more than 1.5, 2) a minimal expression in the embryo (E12.5) of at least 1000 reads and 3) the highest rank. This discriminatory method allowed us to identify the genes Lgi2, Fezf2, Sema3c, Six6, Sox14, Lmo4, Nwd2, Nkx2.1. To have a visuospatial idea of these affected genes, the validation of these results was done by in situ hybridization on E12.5 embryo hypothalamus. We have been able to see an overexpression in the PVN domain for the Lgi2, Fezf2, Sema3c, Lmo4 and Pou3f2 markers. The reduction of expression for Sox14 and Nkx2.1 markers were visible in the basal domain of the hypothalamus, which suggest a non cell autonomous effect of Pou3f2 being overexpressed. The reduction of Six6 couldn’t be consistently visible with repetition. Secondly, a redundant role of OTP and SIM1 seems to occur in the development of the hypothalamus. We created a KO line of the Otp gene by deleting the second exon with CrispR-cas9 and characterized it. We then compared it to the Sim1+/tlz+ line that we already generated in the lab. We were able to confirm our mutation model by seeing a reduction in the expression of crucial markers such as OT, OTP, AVP and TRH. Thirdly, we crossed Otp+/- with Sim1+/tlz+ mice to obtain four different genotypes: wt, Otp+/-, Sim1+/tlz+ and Otp+/- Sim1+/tlz+. Since a redundant aspect has been observed for SIM1 and OTP transcription factors, we were wondering if the obesity phenotype would be worsened by carrying both mutation or not. These mice were weighted every week from 5-week-old up to 6 months old. Food intake has also been measured since the obesity has been reported to be caused by hyperphagia in Sim1 mutant mice. The male mice carrying the double mutation (Otp+/-Sim1+/tlz+) showed a more important weight gain than only Sim1+/tlz+ or Otp+/- mutants, but it was not the case for the female mice. The mice carrying the Otp mutation still got a more important weight gain than the wt mice (females and males). More mice would be necessary to determine if this weight gain is caused by hyperphagia only or if unbalance energy cost is part of the cause.

Sim1

Otp

POU3F2

Hypothalamus

Facteurs de transcription

Noyau paraventriculaire

hyperphagie

équilibre énergétique

ocytocine

vasopressine

CRISPR-Cas9

cascade transcriptionnelle

hybridation in situ

promoteur

embryon de souris

développement.

transcription factors

paraventricular nucleus (PVN)

hyperphagia

transcriptional cascade

in situ hybridization

promotor

mouse embryos

development

Investigation of peptide nucleic acid fluorescence in situ hybridization for diagnosis of ventilator-associated pneumonia in bronchoalveolar lavage specimens

Phillips, Aaron M.

03 January 2014

Indiana University-Purdue University Indianapolis (IUPUI)

QuickFISH

PNA FISH

VAP

BAL

ventilator-associated pneumonia

bronchoalveolar lavage

AdvanDx

diagnosis

Pneumonia -- Prevention

Bronchoalveolar lavage -- Research

Enteral feeding

Artificial respiration -- Complications

Airway extubation

Nosocomial infections -- Transmission

Peptides -- Biotechnology

Nucleic acid probes -- Research

Gastric acid -- Pathophysiology

Wnt signaling in zebrafish fin regeneration : chemical biology using a GSK3β inhibitor

Curtis, Courtney L.

31 July 2014

Indiana University-Purdue University Indianapolis (IUPUI) / Bone growth can be impaired due to disease, such as osteoporosis. Currently, intermittent parathyroid hormone (PTH) treatment is the only approved therapy in the United States for anabolic bone growth in osteoporosis patients. The anabolic effects of PTH treatment are due, at least in part, to modulation of the Wnt/β-catenin pathway. Activation of the Wnt/ β-catenin pathway using a small molecule inhibitor of GSK3β was previously shown to increase markers of bone formation in vitro. Our study utilized a zebrafish model system to study Wnt activated fin regeneration and bone growth. Wnt signaling is the first genetically identified step in fin regeneration, and bony rays are the main structure in zebrafish fins. Thus, zebrafish fin regeneration may be a useful model to study Wnt signaling mediated bone growth. Fin regeneration experiments were conducted using various concentrations of a GSK3β inhibitor compound, LSN 2105786, for different treatment periods and regenerative outgrowth was measured at 4 and 7 days post amputation. Experiments revealed continuous low concentration (4-5 nM) treatment to be most effective at increasing regeneration. Higher concentrations inhibited fin growth, perhaps by excessive stimulation of differentiation programs. In situ hybridization experiments were performed to examine effects of GSK3β inhibitor on Wnt responsive gene expression. Experiments showed temporal and spatial changes on individual gene markers following GSK3β inhibitor treatment. Additionally, confocal microscopy and immunofluorescence labeling data indicated that the Wnt signaling intracellular signal transducer, β-catenin, accumulates throughout GSK3β inhibitor treated tissues. Finally, experiments revealed increased cell proliferation in fin regenerates following LSN 2105786 treatment. Together, these data indicate that bone growth in zebrafish fin regeneration is improved by activating Wnt signaling. Zebrafish Wnt signaling experiments provide a good model to study bone growth and bone repair mechanisms, and may provide an efficient drug discovery platform.

zebrafish, Wnt, regeneration, bone

Bones -- Growth

Bone regeneration

Zebra danio -- Physiology

Wnt genes

Genetic markers

Wnt proteins

Regeneration (Biology)

Gene expression -- Methodology

Fish as laboratory animals -- Research

Fins (Anatomy)

In situ hybridization

Cellular signal transduction

Cell differentiation

Bones -- Diseases

Tissue engineering

Osteoporosis

Biological nutrient removal in SBR technology: from floccular to granular sludge

Coma Bech, Marta

11 May 2011

Biological nutrient removal has been studied and applied for decades in order to remove nitrogen and phosphorus from wastewater. However, more anthropogenic uses and the continued demand for water have forced the facilities to operate at their maximum capacity. Therefore, the goal of this thesis is to obtain more compact systems for nutrient removal from domestic wastewater. In this sense, optimization and long-term stabilization of high volume exchange ratios reactors, treating higher volumes of wastewater, have been investigated. With the same target, aerobic granular sludge was proposed as a reliable alternative to reduce space and increase loading rates in treatment plants. However, the low organic loading rate from low-strength influents (less than 1 Kg COD•m-3d-1) results in slower granular formation and a longer time to reach a steady state. Because of that, different methodologies and operational conditions were investigated in order to enhance granulation and nutrient removal from domestic wastewater. / L’estudi de l’eliminació biològica de nutrients s’ha dut a terme durant dècades. Tot i això, la influencia de l’home i l’augment de la demanda d’aigua han forçat a les instal•lacions a treballar a la seva capacitat màxima. Així, l’objectiu de la tesi és obtenir sistemes més compactes per a l’eliminació de nutrients de les aigües residuals. En aquest sentit, s’ha investigat l’optimització i estabilització de reactors amb alts volums d’intercanvi, tractant més aigua. Amb el mateix objectiu, el fang granular aeròbic va ser proposat com una alternativa fiable per tal de reduir l’espai i incrementar les càrregues de les depuradores. Tot i això, la granulació amb influents de baixa càrrega (menors a 1 Kg dQO•m-3d-1) resulta més lenta i més dificultosa alhora d’obtenir l’estat estacionari. Per aquesta raó es van investigar diferents metodologies i condicions d’operació per tal de millorar la granularció i l’eliminació de nutrients de les aigües urbanes.

Aerobic granular sludge

AGS

Fang granular aeròbic

Lodo granular aeróbico

EDAR

WWTP

Wastewater treatment plants

Enhaced biological phosphorus removal

EBPR

Eliminació biològica de fòsfor

Eliminación biológica de fósforo

Fluorescence in situ hybridization

FISH

SND

Sequencing batch reactor

SBR

Control del reactor seqüencial

Control del reactor secuencial

504

628

Klonierung und Charakterisierung des Interleukin-1beta-Systems im Gehirn von Callithrix jacchus / Cloning and characterization of the interleukin-1beta-system in the brain of Callithrix jacchus

Köster-Patzlaff, Christiane

03 July 2003

No description available.

570 Biowissenschaften, Biologie

Mathematics and Computer Science

Lipopolysaccharid

RT-PCR

in-situ-Hybridisierung

Immunhistologie

Hippocampus

Claustrum

Cortex

IL-1ra

IL-1RI

IL-1RII

Lipopolysaccharid

RT-PCR

in-situ-Hybridization

Immunhistology

Hippocampus

Claustrum

Cortex

IL-1ra

IL-1RI

IL-1RII

42.13 Molekularbiologie

42.60 Zoologie: Allgemeines

42.63 Tierphysiologie

42.84 Mammalia

WA

WF

WH

Regenerationspotenzial CD133+-hämatopoetischer Progenitorzellen der humanen Nabelschnur beim Nierendefekt im Mausmodell / Regenerative potential of human umbilical cord blood derived CD133 positive hematopoietic progenitor cells after kidney injury in a mouse model

Hoffschulte, Birgit

19 August 2009

No description available.

610 Medizin, Gesundheit

Medicine

Xenotransplantation

Ischämie/Reperfusions-Modell

HLA-Färbung

Magnet-aktivierte Zellsortierung (MACS)

Laser-Scanning-Zytometrie

Laser-Mikrodissektion

xenotransplantation

ischemia/reperfusion model

HLA staining

magnetic activated cell sorting (MACS)

laser scanning cytometry

laser microdissection

44.03

44.88

MED 418: Nephrologie

Microbial sulfate reduction in the tissue of the cold-water sponge Geodia barretti (Tetractinellida, Demospongiea) / Mikrobielle Sulfatreduktion im Gewebe des Kaltwasserschwammes Geodia barretti (Tetractinellida, Demospongiae)

Hoffmann, Friederike

06 May 2003

No description available.

550 Geowissenschaften

Mathematics and Computer Science

Porifera

Invertebraten

marin

Norwegische See

boreal

Histologie

Fluroeszenz in situ Hybridisierung

FISH

Einbetten von Gewebe

Heilung

Regeneration

Reproduktion

Sulfatreduktion

sulfatreduzierende Bakterien

Invertebrat-Bakterien-Symbiose

Biogeochemie

Schwefelkreislauf

Sulfatreduktionsrate

Mikroelektrode

porifera

invertebrates

marine

Norwegian Sea

boreal

histology

fluorescence in situ hybridization

FISH

tissue embedding

cicatrisation

regeneration

reproduction

sulfate reduction

sulfate reducing bacteria

invertebrate-microbe symbiosis

biogeochemistry

sulfur cycle

sulfate reduction rate

microelectrode

42.21

42.15

42.21

42.72

38.19

58.30

VU

WB

WH

WN

WR

WY