Development and Functional Characterization of Fetal Lung Organoids

Laube, Mandy, Pietsch, Soeren, Pannicke, Thomas, Thome, Ulrich H., Fabian, Claire

24 March 2023

Preterminfants frequently suffer frompulmonary complications due to a physiological and structural lung immaturity resulting in significant morbidity and mortality. Novel in vitro and in vivo models are required to study the underlying mechanisms of late lung maturation and to facilitate the development of new therapeutic strategies. Organoids recapitulate essential aspects of structural organization and possibly organ function, and can be used to model developmental and disease processes. We aimed at generating fetal lung organoids (LOs) and to functionally characterize this in vitro model in comparison to primary lung epithelial cells and lung explants ex vivo. LOs were generated with alveolar and endothelial cells from fetal rat lung tissue, using a Matrigel-gradient and air-liquid-interface culture conditions. Immunocytochemical analysis showed that the LOs consisted of polarized epithelial cell adhesion molecule (EpCAM)-positive cells with the apical membrane compartment facing the organoid lumen. Expression of the alveolar type 2 cell marker, RT2-70, and the Club cell marker, CC-10, were observed. Na+ transporter and surfactant protein mRNA expression were detected in the LOs. First time patch clamp analyses demonstrated the presence of several ion channels with specific electrophysiological properties, comparable to vital lung slices. Furthermore, the responsiveness of LOs to glucocorticoids was demonstrated. Finally, maturation of LOs induced by mesenchymal stem cells confirmed the convenience of the model to test and establish novel therapeutic strategies. The results showed that fetal LOs replicate key biological lung functions essential for lung maturation and therefore constitute a suitable in vitro model system to study lung development and related diseases.

info:eu-repo/classification/ddc/610

ddc:610

Pro-oxidative and Pro-inflammatory Mechanisms of Brain Injury in Experimental Animal and 3D Cell Culture Model Systems

Cho, Hyung Joon

27 May 2015

The pro-oxidative and pro-inflammatory mechanisms have been implicated in various human diseases including neurological and psychiatric disorders. However, there is only limited information available on the etiology in the progression of neurological damage to brain. The emergence of tissue engineering with the growing interest in mechanistic studies of brain injury now raises great opportunities to study complex physiological and pathophysiological process in vitro. Therefore, the prime goals of this study include: (1) Determination of the molecular and cellular mechanisms responsible for blast- and radiation-induced brain injuries and (2) Development of a three-dimensional (3D) model system in order to mimic in vivo-like microenvironments to further broaden our knowledge in pro-oxidative and pro-inflammatory mechanisms and their cellular responses within 3D constructs. In the first study, we demonstrated that blast exposure induced specific molecular and cellular alterations in pro-oxidative and pro-inflammatory environments in the brain and neuronal loss with adverse behavioral outcome. The results provide evidence that pro-oxidative and pro-inflammatory environments in the brain could play a potential role in blast-induced neuronal loss and behavioral deficits. In the second study, we investigated that fractionated whole-brain irradiation induced specific molecular and cellular alterations in pro-oxidative and pro-inflammatory environments in the brain along with elevation of reactive oxygen species (ROS)-generating protein (NOX-2) and microglial activation. Additionally, the contribution of NOX-2 in fractionated whole-brain radiation-induced oxidative stress was observed by dramatic amelioration of ROS generation after pharmacological inhibition of NOX-2. These results support that NOX-2 may play a pivotal role in fractionated whole-brain radiation-induced pro-oxidative and pro-inflammatory pathways in mouse brain. In the third study, we developed an in vitro 3D experimental model of brain inflammation by encapsulating microglia in collagen hydrogel with computational analysis of 3D constructs. The results indicated that our newly developed in vitro 3D model system provides a more physiologically relevant environment to mimic in vivo responses. In conclusion, these data may be beneficial in defining a cellular and molecular basis of pathophysiological mechanisms of brain injuries. Furthermore, it may provide new opportunities for preventive and therapeutic interventions for patients with brain injuries and associated neurological disorders. / Ph. D.

Oxidative Stress

Inflammation

Blast-induced Brain Injury

Radiation-induced Brain Injury

Transformação genética de laranjeira doce com genes da via biossintética de carotenoides / Functional analysis of genes of the carotenoid biosynthetic pathway in sweet orange

Pinheiro, Thaísa Tessutti

03 June 2014

Plantas de Citrus regeneradas de tecidos juvenis demandam um longo período para a análise do fenótipo resultante em flores ou frutos. Este trabalho apresenta o mutante espontâneo de florescimento precoce de laranja doce, denominado \'x11\', como modelo para estudos de genômica funcional de Citrus. As frutas cítricas são ricas em carotenoides, pigmentos que possuem grande valor nutricional, como pró-vitamina A (?- ou ?-caroteno). Estudos de genômica funcional envolvendo genes da via biossintética dos carotenoides terão resultados rapidamente obtidos utilizando-se variedades com florescimento e frutificação precoce, como a laranjeira doce mutante \'x11\'. A laranjeira doce \'Sanguínea-de-Mombuca\' (SM) é uma variedade de polpa vermelha que acumula licopeno na polpa dos frutos, podendo ser considerada uma importante ferramenta no estudo da acumulação de carotenoides nos frutos de laranjeiras. Desta maneira, o objetivo deste estudo foi estabelecer a laranjeira \'x11\' como planta-modelo em experimentos de transformação genética visando estudos de genômica funcional dos genes PSY (fitoeno sintase), PDS (fitoeno desaturase), CRTISO (carotenoide isomerase), LCY-b (licpeno ?-ciclase) e ?-caroteno hidroxilase (HYb), envolvidos na biossíntese de carotenoides e utilizar a laranjeira SM como ferramenta no entendimento da acumulação dos carotenoides nos frutos de Citrus. Plantas de laranjeira \'x11\' foram transformadas com promotor de expressão preferencial para órgãos reprodutivos de Citrus controlando a expressão de gene repórter (gusA) para a análise da tecido especificidade. Foi realizada a otimização do protocolo de transformação genética de segmentos de epicótilo de laranjeira \'x11\' via Agrobacterium. A eficiência de transformação média foi de 18,6%, mas atingiu 29,6% no protocolo otimizado. Das 270 brotações positivas, cinco foram microenxertadas e aclimatizadas. Quatro dessas plantas exibiram as primeiras flores em três meses após o estabelecimento ex vitro, e a outra, dois meses mais tarde, independentemente da época do ano. A coloração histoquímica da atividade do gene gusA foi realizada em segmentos de caule, flores e frutos de plantas transgênicas aclimatizadas, com 5-7 meses de idade, confirmando a expressão constitutiva do gene gusA nesses órgãos. As plantas transformadas com a construção para o teste do promotor de expressão preferencial para órgãos reprodutivos de Citrus continuam em fase de desenvolvimento. Em seguida foi realizada a transformação genética de laranjeira \'x11\' para a superexpressão dos genes PDS e LCY-b1 e para a superexpressão do gene LCY-b1 e HYb em laranjeira SM. Também foi realizada a transformação genética de \'x11\' para o silenciamento do gene CRTISO e HYb e também para o silenciamento do gene CRTISO, em SM. A quantificação da expressão do gene-alvo em tecido foliar foi correlacionada ao número de cópias do cisgene inseridos em cada planta, revelando que o nível de expressão gênica não foi diretamente ligado ao número de cópias inseridas no genoma. Uma planta de laranjeira \'x11\' superexpressando o gene LCY-b1 frutificou e foi realizada a análise do perfil de carotenoides totais em relação ao fruto de uma planta não transformada. Neste evento houve aumento no teor de carotenoides totais e xantofilas, indicando o potencial da manipulação dos genes codificadores de enzimas da via biossíntese de carotenoides para alterações quantitativas e qualitativas destes pigmentos / Considering the perennial developmental phase of Citrus, plants regenerated from juvenile tissues require long period for analysis of the resulting phenotype in flowers or fruits. Herein, we present the spontaneous sweet orange mutant named \'x11\', as a model plant for functional genomics studies in Citrus due to the remarkable feature of early-flowering. Citrus fleshy fruits are rich in carotenoids which are pigments that have great nutritional value, such as pro-vitamin A (?- or ?-carotene). Functional genomics studies involving genes related to carotenoids biosynthesis pathway can be rapid generated by using the early flowering mutant, \'x11\' in sweet orange background. The fleshy fruit from the sweet orange \'Sanguínea-de-Mombuca\' (SM) has a red pulp due to accumulation lycopene that may be considered an important tool to investigate the accumulation of carotenoids in sweet orange fruits. Therefore, the aim of this study was to establish the orange mutant \'x11\'as model plants for genetic transformation and functional genomics analysis of key regulatory genes PSY (phytoene synthase), PDS (phytoene desaturase), CRTISO (carotenoid isomerase), LCY-b1 (licopene ?-cyclase) and ?-carotene hydroxylase (HYb) involved in the biosynthesis of carotenoids and to use the sweet orange SM as a tool in understanding the accumulation of carotenoids in sweet orange fruits. The mutant plants \'x11\' were transformed with gene reporter (gusA) under control of specific promoter for reproductive organs in Citrus for the tissue specificity analysis. We report a procedure for efficient regeneration and transformation using epicotyl segment explants of \'x11\' and Agrobacterium tumefaciens as a proof-of-concept. The average transformation efficiency was 18.6%, but reached 29.6% in the best protocol tested. Among 270 positive shoots, five were micrografted and acclimatized. Four of these plants exhibited the first flowers within three months after ex vitro establishment, and the other, two months later, regardless the period of the year. Transgenic plants harboring specific promoter for reproductive organs in Citrus are still under development. We transformed \'x11\' for overexpression of PDS or LCY-b1 genes, and to overexpress LCY-b1 or HYb in SM sweet orange. \'x11\' was transformed to silence CRTISO or HYb , and CRTISO gene in SM sweet orange. Then, quantification of target gene expression in leaf tissue was performed by correlating this information with the number of copies of cisgene inserted into each plant. According to the results, it is suggested that the level of gene expression is not directly linked to the number of copies inserted into the genome.One transgenic plant of \'x11\' overexpressing LCY-b1 produced flowers and fruits and the carotenoid profile analysis indicated an increased in content of total carotenoids and, especially, xanthophylls, clearly indicating the potential to manipulate expression of genes encoding enzymes of the carotenoid biosynthetic pathway to obtain qualitatively and quantitatively changes of these pigments

Biossíntese

Biosynthesis

Carotenoid

Carotenoide

Cisgenia

Cisgeny

Citrus

Citrus

Flor

Flower

Fruit

Fruto

Gene

Gene

Genômica funcional

Genomics functional

Laranja

Model system

Sistema modelo

Sweet Orange

Transgenic

Transgênico

Developing an optimal method for producing a tearless onion

Kamoi, T.

January 2008

People experience the irritating tearing and burning sensation of lachrymatory factor (LF, propanthial S-oxide) when cutting or chopping onion bulbs. LF is produced by lachrymatory factor synthase (LFS) specifically from 1-propenyl sulfenic acid, a breakdown product of trans-1-propenyl-L-cysteine sulfoxide (1-PRENCSO) by alliinase. This thesis describes strategies to produce a tearless onion by using RNA interference (RNAi) silencing. To determine whether a gene silencing cassette can silence lfs gene transcripts from onion (Allium cepa L.), a crop recalcitrant to genetic transformation, a gene silencing assessment system was developed by using a model plant as a host for the gene of interest. Tobacco (Nicotiana tabacum) plants transgenic for LFS enzyme activity from onion were first produced by introducing a CaMV 35S-onion-lfs gene construct. These plants were then subjected to a second transformation with an RNAi construct directed against the lfs gene sequence. LFS enzyme activity assay showed that the transgenic plants, containing both the lfs gene and the RNAi construct, had significantly reduced LFS activity. This observation was supported by Western analysis for the LFS protein and further validated by quantitative RT-PCR analysis that demonstrated a significant reduction in the lfs transcript level in the dual transformants. This work demonstrated that the RNAi construct is a suitable candidate for the development of a tearless onion. This model plant RNAi system has wide reaching applications for assessment and targeting of plant secondary pathway genes, from poorly studied or recalcitrant plant species, that are important in pharmacological, food and process industries. The functional RNAi vector identified in the model system was transformed into onion. Endogenous lfs transcript levels were successfully reduced by up to 43-fold in six transgenic lines. In consequence, LFS enzyme activity was decreased by up to 1573-fold and this observation was supported by Western analysis for the LFS protein. Furthermore, the production of the deterrent LF upon tissue disruption was reduced up to 67-fold. Subjective olfactory assessment of silenced lines indicated that the pungent odour given off by the leaf and bulb material was much reduced compared with that of non-transgenic counterparts, and that this was replaced by a sweeter milder onion odour. A novel colorimetric assay demonstrated that this silencing had shifted the 1-PRENCSO breakdown pathway so that by reducing LFS protein, more 1-propenyl sulfenic acid was converted into di-1-propenyl thiosulfinate. A consequence of the raised thiosulfinates levels was a marked increase in the downstream production of a non-enzymatically produced zwiebelane isomer that has never previously been identified, and other volatile compounds, di-1-propenyl disulfides and 2-mercapto-3,4-dimethyl-2,3-dihydrothiophenes, which had previously been reported either in small amounts or had not been detected in onions. These raised volatile sulfur compounds provide an explanation for the unique flavour notes of the LF reduced onion and are predicted to have health benefits akin to those found in garlic. These results demonstrated that silencing of LFS enzyme activity by introducing an RNAi construct directed against the lfs gene sequence simultaneously reduced levels of the deterrent LF and increased the desirable thiosulfinates in onions.

onion

lachrymatory factor synthase

propanthial S-oxide

RNA interference

gene silencing

model system

colorimetric assay

thiosulfinates

zwiebelane isomer

disulfides

dihydrothiophenes

Exploiting and exploring the interactions between microRNA-122 and Hepatitis C virus

2014 September 1900

Hepatitis C virus (HCV) is a single-stranded plus-sense RNA virus that is transmitted by blood-to-blood contact, and infects the human liver. HCV has a unique dependence on the liver-specific microRNA miR-122, where miR-122 binds the 5´ un-translated region of the viral RNA at two tandem sites and increases viral RNA abundance. The mechanisms of augmentation are not yet fully understood, but the interaction is known to stabilize the viral RNA, increase translation from the viral internal ribosomal entry site (IRES), and result in increased viral yield. In an attempt to create a small animal model for HCV, we added miR-122 to mouse cell lines previously thought non-permissive to HCV, which rendered these cells permissive to the virus, additionally showing that miR-122 is one of the major determinants of HCV hepatotropism. We found that some wild-type and knockout mouse cell lines – NCoA6 and PKR knockout embryonic fibroblasts – could be rendered permissive to transient HCV sub-genomic, but not full-length, RNA replication upon addition of miR-122, and that other wild-type and knockout cell lines cannot be rendered permissive to HCV replication by addition of miR-122. These knockout cell lines demonstrated varying permissiveness phenotypes between passages and isolates and eventually completely lost permissiveness, and we were unable to achieve sub-genomic RNA replication in PKR knockout primary hepatocytes. Knockdown of NCoA6 and PKR in Huh7.5 cells did not substantially impact sub-genomic replication, leading us to conclude that there are additional factors within the cell lines that affect their permissiveness for HCV replication such as epigenetic regulation during passage or transformation and immortalization. We also added miR-122 to Hep3B cells, a human hepatoma cell line lacking expression of miR-122 and previously thought to be non-permissive to HCV replication. Added miR-122 rendered the cells as highly permissive to HCV replication as the Huh7-derived cell lines commonly used to study the virus. In these cells, we were also able to observe miR-122-independent replication of sub-genomic HCV RNA. This was verified by use of a miR-122 antagonist that had no impact on the putative miR-122-independent replication, and by mutating the miR-122 binding sites to make them dependent on a single nucleotide-substituted microRNA. This replication in the absence of miR-122 was not detected in full-length HCV RNA, but was detectable using a bi-cistronic full-length genomic replicon, suggesting that the addition of a second IRES in sub-genomic and full-genomic replicons altered replication dynamics enough to allow detectable RNA replication without miR-122 binding. Because miR-122 has been implicated in protecting the viral RNA from destabilization and degradation by Xrn1, the main cytoplasmic 5´ to 3´ RNA exonuclease, we employed our miR-122-independent system to test this miR-122-mediated protection. We verified that miR-122 functions to protect the viral RNA from Xrn1, but this was insufficient to account for the overall impact of miR-122 on replication, meaning that miR-122 has further functions in the virus’ life cycle. We showed that the effect of miR-122 on translation is due to stabilization of the RNA by protecting it from Xrn1, through binding at both sites. We further evaluated the role of each miR-122 binding site (S1 and S2) in the virus life cycle, and found that binding at each site contributes equally to increasing viral RNA replication, while binding at both sites exerts a co-operative effect. Finally, we determined that binding of miR-122 at site S2 is more important for protection from Xrn1, suggesting that miR-122 binding at S1 is more important for the additional functions of miR-122 in enhancing HCV RNA accumulation. Altogether, we have shown that miR-122 is partially responsible for the hepatotropic nature of Hepatitis C virus, and that supplementation with this microRNA can render non-permissive cells permissive to viral replication. We have also identified and confirmed replication of both sub-genomic and full-length HCV RNA in the absence of miR-122. Finally, we have characterized the impact of the host RNA exonuclease Xrn1 on the HCV life cycle, and determined the roles of each miR-122 binding site in shielding the viral RNA from this host restriction factor.

Hepatitis C virus

HCV

microRNA

miR-122

Hep3B

murine embryonic fibroblast

MEF

virus-host interactions

animal model

model system

Xrn1

virus replication

Dissection de la fonction du RCPG d'adhésion BAI3 dans la fusion des myoblastes

Hamoud, Noumeira

03 1900

No description available.

Myogenesis

Myotube formation

GPCR signaling

cell-cell fusion

Model system

Myogenèse

Formation de myotubes

Fusion cellules-cellules

RCPG

Modèles expérimentaux

Transformação genética de laranjeira doce com genes da via biossintética de carotenoides / Functional analysis of genes of the carotenoid biosynthetic pathway in sweet orange

Thaísa Tessutti Pinheiro

03 June 2014

Plantas de Citrus regeneradas de tecidos juvenis demandam um longo período para a análise do fenótipo resultante em flores ou frutos. Este trabalho apresenta o mutante espontâneo de florescimento precoce de laranja doce, denominado \'x11\', como modelo para estudos de genômica funcional de Citrus. As frutas cítricas são ricas em carotenoides, pigmentos que possuem grande valor nutricional, como pró-vitamina A (?- ou ?-caroteno). Estudos de genômica funcional envolvendo genes da via biossintética dos carotenoides terão resultados rapidamente obtidos utilizando-se variedades com florescimento e frutificação precoce, como a laranjeira doce mutante \'x11\'. A laranjeira doce \'Sanguínea-de-Mombuca\' (SM) é uma variedade de polpa vermelha que acumula licopeno na polpa dos frutos, podendo ser considerada uma importante ferramenta no estudo da acumulação de carotenoides nos frutos de laranjeiras. Desta maneira, o objetivo deste estudo foi estabelecer a laranjeira \'x11\' como planta-modelo em experimentos de transformação genética visando estudos de genômica funcional dos genes PSY (fitoeno sintase), PDS (fitoeno desaturase), CRTISO (carotenoide isomerase), LCY-b (licpeno ?-ciclase) e ?-caroteno hidroxilase (HYb), envolvidos na biossíntese de carotenoides e utilizar a laranjeira SM como ferramenta no entendimento da acumulação dos carotenoides nos frutos de Citrus. Plantas de laranjeira \'x11\' foram transformadas com promotor de expressão preferencial para órgãos reprodutivos de Citrus controlando a expressão de gene repórter (gusA) para a análise da tecido especificidade. Foi realizada a otimização do protocolo de transformação genética de segmentos de epicótilo de laranjeira \'x11\' via Agrobacterium. A eficiência de transformação média foi de 18,6%, mas atingiu 29,6% no protocolo otimizado. Das 270 brotações positivas, cinco foram microenxertadas e aclimatizadas. Quatro dessas plantas exibiram as primeiras flores em três meses após o estabelecimento ex vitro, e a outra, dois meses mais tarde, independentemente da época do ano. A coloração histoquímica da atividade do gene gusA foi realizada em segmentos de caule, flores e frutos de plantas transgênicas aclimatizadas, com 5-7 meses de idade, confirmando a expressão constitutiva do gene gusA nesses órgãos. As plantas transformadas com a construção para o teste do promotor de expressão preferencial para órgãos reprodutivos de Citrus continuam em fase de desenvolvimento. Em seguida foi realizada a transformação genética de laranjeira \'x11\' para a superexpressão dos genes PDS e LCY-b1 e para a superexpressão do gene LCY-b1 e HYb em laranjeira SM. Também foi realizada a transformação genética de \'x11\' para o silenciamento do gene CRTISO e HYb e também para o silenciamento do gene CRTISO, em SM. A quantificação da expressão do gene-alvo em tecido foliar foi correlacionada ao número de cópias do cisgene inseridos em cada planta, revelando que o nível de expressão gênica não foi diretamente ligado ao número de cópias inseridas no genoma. Uma planta de laranjeira \'x11\' superexpressando o gene LCY-b1 frutificou e foi realizada a análise do perfil de carotenoides totais em relação ao fruto de uma planta não transformada. Neste evento houve aumento no teor de carotenoides totais e xantofilas, indicando o potencial da manipulação dos genes codificadores de enzimas da via biossíntese de carotenoides para alterações quantitativas e qualitativas destes pigmentos / Considering the perennial developmental phase of Citrus, plants regenerated from juvenile tissues require long period for analysis of the resulting phenotype in flowers or fruits. Herein, we present the spontaneous sweet orange mutant named \'x11\', as a model plant for functional genomics studies in Citrus due to the remarkable feature of early-flowering. Citrus fleshy fruits are rich in carotenoids which are pigments that have great nutritional value, such as pro-vitamin A (?- or ?-carotene). Functional genomics studies involving genes related to carotenoids biosynthesis pathway can be rapid generated by using the early flowering mutant, \'x11\' in sweet orange background. The fleshy fruit from the sweet orange \'Sanguínea-de-Mombuca\' (SM) has a red pulp due to accumulation lycopene that may be considered an important tool to investigate the accumulation of carotenoids in sweet orange fruits. Therefore, the aim of this study was to establish the orange mutant \'x11\'as model plants for genetic transformation and functional genomics analysis of key regulatory genes PSY (phytoene synthase), PDS (phytoene desaturase), CRTISO (carotenoid isomerase), LCY-b1 (licopene ?-cyclase) and ?-carotene hydroxylase (HYb) involved in the biosynthesis of carotenoids and to use the sweet orange SM as a tool in understanding the accumulation of carotenoids in sweet orange fruits. The mutant plants \'x11\' were transformed with gene reporter (gusA) under control of specific promoter for reproductive organs in Citrus for the tissue specificity analysis. We report a procedure for efficient regeneration and transformation using epicotyl segment explants of \'x11\' and Agrobacterium tumefaciens as a proof-of-concept. The average transformation efficiency was 18.6%, but reached 29.6% in the best protocol tested. Among 270 positive shoots, five were micrografted and acclimatized. Four of these plants exhibited the first flowers within three months after ex vitro establishment, and the other, two months later, regardless the period of the year. Transgenic plants harboring specific promoter for reproductive organs in Citrus are still under development. We transformed \'x11\' for overexpression of PDS or LCY-b1 genes, and to overexpress LCY-b1 or HYb in SM sweet orange. \'x11\' was transformed to silence CRTISO or HYb , and CRTISO gene in SM sweet orange. Then, quantification of target gene expression in leaf tissue was performed by correlating this information with the number of copies of cisgene inserted into each plant. According to the results, it is suggested that the level of gene expression is not directly linked to the number of copies inserted into the genome.One transgenic plant of \'x11\' overexpressing LCY-b1 produced flowers and fruits and the carotenoid profile analysis indicated an increased in content of total carotenoids and, especially, xanthophylls, clearly indicating the potential to manipulate expression of genes encoding enzymes of the carotenoid biosynthetic pathway to obtain qualitatively and quantitatively changes of these pigments

Biossíntese

Carotenoide

Cisgenia

Citrus

Flor

Fruto

Gene

Genômica funcional

Laranja

Sistema modelo

Transgênico

Biosynthesis

Carotenoid

Cisgeny

Citrus

Flower

Fruit

Gene

Genomics functional

Model system

Sweet Orange

Transgenic

Aplikace systémových přístupů na zavedení data warehouse nástroje / Application of system approach to the delivery of data warehouse tool

Šubrt, Radek

January 2011

This diploma thesis is focused on the application of a system approach, which was configured by the author. Configured approach was used to analyze project of implementation of data warehouse tool. Dynamics of the project delivery system was shown by causal loop diagram and then by system dynamics model. Thesis defined and used terms like system, system complexity, system approach, system approach configuration, causal loop diagram, system dynamics model, system archetype of shifting the burden, data warehouse and its definition against a database definition, project, project organizational structures, methods and their necessity in implementation of information systems projects, feasibility of the information system projects and problems with measurement of project performance. Time-proportional simulation of system dynamics model quantified effects of factors and also quantified different results of project implementation approaches. Based on the analyzed project was provided a brief general recommendations for information systems projects.

Ein Beitrag zur makroskopischen Simulation von Passagierströmen zwischen kooperierenden Flughäfen unter Nutzung des SYSTEM DYNAMICS Zuganges nach Forrester

Mühlhausen, Thorsten

22 December 1999

Der stetig steigende Flugverkehr führt zu Kapazitätsengpässen an vielen Großflughäfen. Die Möglichkeit des Ausbaus ist häufig aufgrund von Arealmangel und Widerstand aus der Bevölkerung (zumeist durch Umweltgesichtspunkte motiviert) nicht realisierbar. Ein Ausweg bietet hier die Kooperation mehrerer Flughäfen. So kann ein in der Nähe eines Großflughafens angesiedelter Regionalflughafen als zusätzliche Runwaygenutzt werden. Ausschlaggebend hierbei sind die landseitigen Anbindungen beider Flughäfen. Beide müssen zusammen annähernd wie ein Flughafen operieren. Der Optimierung dieses Systems kooperierender Flughäfen widmet sich die vorliegende Arbeit. Es werden zwei Szenarien näher untersucht und bewertet: Konventionelle S-Bahn-Verbindung unter Ausnutzung der vorhandenen Infrastruktur und mit einem fixen Fahrplan (traditioneller Betrieb) Verbindung unter Nutzung einer vollautomatischen Bahn mit bedarfsabhängiger Anpassung der Taktrate Die Modellierung erfolgt hierbei durch eine makroskopische Simulation auf der Basis des SYSTEM DYNAMICS Zugangs nach Forrester. Dieser zeichnet sich besonders durch seine prozessnahe Darstellung aus. In dieser Arbeit wird die Anwendbarkeit von SYSTEM DYNAMICS auf die Modellierung von Passagierströmen an Verkehrsknoten nachgewiesen, die Passagierverzögerung bei der Verknüpfung von Flughäfen ermittelt und der Ressourcenverbrauch, d.h. der Bedarf an Betriebsmitteln für die Verbindung bestimmt. / Steadily increasing air traffic leads to capacity problems at many major airports. In most cases it is not possible to enlarge the airport due to lack of area or resistance of the population (mainly motivated by environmental aspects). One way out is the cooperation of airports. It can be possible to use a smaller airport in the vicinity of a major airport as an additional runway. In this case the land-side connections between both airports are very important. The two airports have to operate like one big airport. This work deals with the optimization of the system of cooperating airports. Two scenarios are analyzed and rated in more detail: Conventional railway connection with utilization of existing infrastructure and with a fixed time table (traditional operational regime) Connection with an automated people mover with demand control schedule For macroscopic modeling the SYSTEM DYNAMICS approach by Forrester is used. The main feature is a very good real world representation. This work shows the applicability of SYSTEM DYNAMICS for modeling passenger flows at traffic junctions, calculates the passenger delay, which occurs between connected airports and specifies the consumption of resources, i.e. equipment necessary for the connection.

info:eu-repo/classification/ddc/41

ddc:41

Economic model of mine closure and its potential for economic transformation

Toni

07 April 2015

In Indonesia, the various mining commodities and the amount of resources and reserves are promising, as evidence there are numerous large-scale mining companies and small-scale mines in operation. In 2014 there were 41 companies that held the CoW (mineral contract of work) and 13 companies active in production; and 76 CCoW (coal contract of work) holders, and 57 companies active in production. As well as this, there are more than a thousand small-scale mining companies active for mining commodities. However, mining commodities provide a resource that is not renewable. This will potentially lead to prolonged problems when mining companies do not adhere to good mining practices, particularly in the closing stages of the mine. Mine closure is the final stage in the process of mining activity. In certain circumstances, closure activities can take a long time and of course can have huge costs. In fact, at this stage, the company is no longer making profit, only incurring costs for the project closure. To prevent problems that may arise after the mine is closed, such as abandoned post-mining land, and the bankruptcy of the company at the end of mining operations, etc., then through specific rules, ie rules of the Minister of Energy and Mineral Resources No. 18 of 2008, the mining company in Indonesia must provide a certain amount of money as a financial guarantee to finance the planned closure project; it must be approved by the government before entering this phase. However, problems are encountered in practice. The government may become overloaded because they have to quickly make a decision on the closure plan submitted by the company. So a tool is needed that can be used to assess the feasibility as soon as the mine closure plan is proposed by a company, these tools can provide an overview and a variety of options for decision making. In this dissertation methodology was developed to create a systems dynamic model of mine closure. The model developed can be applied to a variety of mining methods and for various mining commodities. The model can be used to determine the closure costs, to choose the closure project-financing scenario, and up to micro and macro economic analysis of mining activities in the region. In the case studies conducted in this dissertation, the best scenario of the mine closure planning is to include the everlasting fund in the form of time deposits, and convert the post-mining land for agriculture. The amount of deposit money is about USD 358,986,500 should be spare at the end of mine production, and the total of mine closure cost to be approximately USD 440,757,384. Agriculture, the economic sector as a substitute for the mining sector, the added value to the GRDP (Gross Regional Domestic Product) is about 0.25 % / a for the province, and 1.68 % for the regency, but the contribution of the mining sector to GRDP was 30% / a at province scale, and 90% / a at regency scale. So that the substitution value is less significant to GRDP growth. However, this scenario is the best scenario among others, due to consideration is the certainty of ecological and economic sustainability. it is the best goal of corporate social responsibility to the environment in the post- mining land.

info:eu-repo/classification/ddc/624

ddc:624