Spelling suggestions: "subject:"promotor."" "subject:"oromotor.""
171 |
Charakterizace promotorových oblastí genů HGSNAT a GBA, a příspěvek ke studiu patogeneze MPS IIIC a Gaucherovy choroby / Characterization of promoter regions of HGSNAT and GBA genes, and a contribution to the study of pathogenesis of MPS IIIC and Gaucher diseaseRichtrová, Eva January 2014 (has links)
Pathogenesis of mucopolysaccharidosis type IIIC (MPS IIIC) and Gaucher disease has not been yet fully clarified, and the causes of phenotypical variability between the patients with the same genotype in Gaucher disease remain obscure. Because the variants in the regulatory regions of genes can cause phenotypical differences mentioned above, I have studied promoter regions of HGSNAT and GBA genes mutated in these lysosomal disorders. I have shown that there is an alternative promoter of GBA (P2). Additional studies were aimed to elucidate possible physiological functions of P2, and its possible role in the pathogenesis of Gaucher disease. I have found that P2 is not tissue specific, and that its variants do not influence the variability of phenotype in Gaucher patients with the same genotype. P2 is used differentially neither during the differentiation of monocytes to macrophages nor in macrophages from controls and Gaucher patients, in whom there is a prominent storage only in cells of macrophage origin. We have thus not found any changes that would suggest a role for P2 in the pathogenesis of Gaucher disease. I have characterized the promoter region of HGSNAT and shown that the binding of Sp1 transcription factor is important for its expression. Sequence variants found in HGSNAT promoter in...
|
172 |
Mechanismy regulace exprese genů pro ornitin transkarbamylázu a beta-glukocerebrosidázu a jejich význam v diagnostice / Regulatory mechanisms of ornithin transcarbamylase and beta-glucocerebrosidase gene expression and their relevance to diagnosticsLukšan, Ondřej January 2014 (has links)
5 Abstract Definitive diagnosis of inherited metabolic disorders commonly depends on the measurement of enzyme activity (which is often complicated) and/or molecular genetic testing. Yet even the standard mutation analysis can bring false negative results in the case of gross chromosomal rearrangements or incorrect regulation of gene expression due to the mutations in regulatory regions. In the present study I focused on characterization of complex mutations affecting the gene encoding ornithin transcarbamylase (OTC) followed by studies of regulatory regions of OTC and GBA (the gene encoding β-glucocerebrosidase). In the first study we identified 14 novel mutations including three large deletions in a cohort of 37 patients with OTC deficiency (OTCD). Subsequently we evaluated clinical significance of all these mutations. We also found a heterozygote carrying a hypomorphic mutation and manifesting OTCD most likely due to unfavorable X-inactivation which was observed independently in three different peripheral tissues. In order to evaluate the clinical significance of a promoter variation c.-366A>G found in a family with mild OTCD we identified three alternative transcription start sites (TSSs) of human OTC and delimited the promoter. We also found a distal enhancer and performed functional analysis of both...
|
173 |
Charakterizace role SPINK 6 v epidermis za použití transgenních modelů / Characterization of the role of SPINK 6 in the epidermis using transgenic modelsBuryová, Halka January 2011 (has links)
Epidermal homeostasis, including proper turnover of keratinocytes, plays important role in the barrier function and serine proteases and their inhibitors are the key players. Activated proteases cleave desmosomes in uppermost layer and thus shed the cells from the epidermal surface. Therefore the serine protease inhibitors are secreted in lower epidermal layers to prevent premature activation of proteases and consequent disruption of epidermal barrier. The most studied inhibitors in epidermis belong to Serine proteases inhibitors Kazal-type family (SPINK). This diploma thesis is aimed to investigate function of murine SPINK6 in epidermal compartment in vivo. To achieve this, the transgenic mice overexpressing mSPINK6 under modified human involucrin promoter was generated. Two of five transgenic lines exhibited higher expression of mSPINK6 at mRNA and protein levels. The mSPINK6 transgenic mice are viable with no apparent phenotype. The small but in most cases not significant differences were observed on microscopic level among mSPINK6 transgenic and wild type animals In conclusion, this work showed that mSPINK6 does not play major role in skin homeostasis but gains significant importance under specific challenges of epidermal barrier. Therefore mSPINK6 transgenic mice, in combination with other deletion or...
|
174 |
Charakterizace promotorových oblastí genů HGSNAT a GBA, a příspěvek ke studiu patogeneze MPS IIIC a Gaucherovy choroby / Characterization of promoter regions of HGSNAT and GBA genes, and a contribution to the study of pathogenesis of MPS IIIC and Gaucher diseaseRichtrová, Eva January 2014 (has links)
Pathogenesis of mucopolysaccharidosis type IIIC (MPS IIIC) and Gaucher disease has not been yet fully clarified, and the causes of phenotypical variability between the patients with the same genotype in Gaucher disease remain obscure. Because the variants in the regulatory regions of genes can cause phenotypical differences mentioned above, I have studied promoter regions of HGSNAT and GBA genes mutated in these lysosomal disorders. I have shown that there is an alternative promoter of GBA (P2). Additional studies were aimed to elucidate possible physiological functions of P2, and its possible role in the pathogenesis of Gaucher disease. I have found that P2 is not tissue specific, and that its variants do not influence the variability of phenotype in Gaucher patients with the same genotype. P2 is used differentially neither during the differentiation of monocytes to macrophages nor in macrophages from controls and Gaucher patients, in whom there is a prominent storage only in cells of macrophage origin. We have thus not found any changes that would suggest a role for P2 in the pathogenesis of Gaucher disease. I have characterized the promoter region of HGSNAT and shown that the binding of Sp1 transcription factor is important for its expression. Sequence variants found in HGSNAT promoter in...
|
175 |
Mechanismy regulace exprese genů pro ornitin transkarbamylázu a beta-glukocerebrosidázu a jejich význam v diagnostice / Regulatory mechanisms of ornithin transcarbamylase and beta-glucocerebrosidase gene expression and their relevance to diagnosticsLukšan, Ondřej January 2014 (has links)
5 Abstract Definitive diagnosis of inherited metabolic disorders commonly depends on the measurement of enzyme activity (which is often complicated) and/or molecular genetic testing. Yet even the standard mutation analysis can bring false negative results in the case of gross chromosomal rearrangements or incorrect regulation of gene expression due to the mutations in regulatory regions. In the present study I focused on characterization of complex mutations affecting the gene encoding ornithin transcarbamylase (OTC) followed by studies of regulatory regions of OTC and GBA (the gene encoding β-glucocerebrosidase). In the first study we identified 14 novel mutations including three large deletions in a cohort of 37 patients with OTC deficiency (OTCD). Subsequently we evaluated clinical significance of all these mutations. We also found a heterozygote carrying a hypomorphic mutation and manifesting OTCD most likely due to unfavorable X-inactivation which was observed independently in three different peripheral tissues. In order to evaluate the clinical significance of a promoter variation c.-366A>G found in a family with mild OTCD we identified three alternative transcription start sites (TSSs) of human OTC and delimited the promoter. We also found a distal enhancer and performed functional analysis of both...
|
176 |
Physico-Chemical Processes during Reactive Paper Sizing with Alkenyl Succinic Anhydride (ASA) / Physikochemische Prozesse während der Reaktivleimung mit Alkenyl-Bernsteinsäure-Anhydrid (ASA)Porkert, Sebastian 27 February 2017 (has links) (PDF)
Sizing (hydrophobization) is one of the most important process steps within the added-value chain of about 1/3rd of the worldwide produced paper & board products. Even though sizing with so-called reactive sizing agents, such as alkenyl succinic anhydride (ASA) was implemented in the paper industry decades ago, there is no total clarity yet about the detailed chemical and physical mechanisms that lead to their performance. Previous research was carried out on the role of different factors influencing the sizing performance, such as bonding between ASA and cellulose, ASA hydrolysis, size revision as well as the most important interactions with stock components, process parameters and additives during the paper making process. However, it was not yet possible to develop a holistic model for the explanation of the sizing performance given in real life application. This thesis describes a novel physico-chemical approach to this problem by including results from previous research and combining these with a wide field of own basic research and a newly developed method that allows tracing back the actual localization of ASA within the sheet structure.
The carried out measurements and trial sets for the basic field of research served to evaluate the stock and process parameters that most dominantly influence the sizing performance of ASA. Interactions with additives other than retention aids were not taken into account. The results show that parameters, such as the content of secondary fibers, the degree of refining, the water hardness as well as the suspension conductivity, are of highest significance. The sample sets of the trials with the major impacting parameters were additionally analyzed by a newly developed localization method in order to better understand the main influencing factors.
This method is based on optical localization of ASA within the sheet structure by confocal white light microscopy. In order to fulfill the requirements at magnification rates of factor 100 optical zoom, it was necessary to improve the contrast between ASA and cellulose. Therefore, ASA was pretreated with an inert red diazo dye, which does not have any impact on neither the sizing nor the handling properties of ASA. Laboratory hand sheets that were sized with dyed ASA, were analyzed by means of their sizing performance in correlation to measurable ASA agglomerations in the sheet structure. The sizing performance was measured by ultrasonic penetration analysis. The agglomeration behavior of ASA was analyzed automatically by multiple random imaging of a sample area of approx. 8650 µm² with a minimum resolution for particles of 500 nm in size. The gained results were interpreted by full factorial design of experiments (DOE). The trials were carried out with ASA dosages between 0% and 0.8% on laboratory hand sheets, made of 80% bleached eucalyptus short fiber kraft pulp and 20% northern bleached softwood kraft pulp, beaten to SR° 30, produced with a RDA sheet former at a base weight of 100 g/m² oven dry.
The results show that there is a defined correlation between the ASA dosage, the sizing performance and the number and area of ASA agglomerates to be found in the sheet structure. It was also possible to show that the agglomeration behavior is highly influenced by external factors like furnish composition and process parameters. This enables a new approach to the explanation of sizing performance, by making it possible to not only examine the performance of the sizing agent, but to closely look at the predominant position where it is located in the sheet structure. These results lead to the explanation that the phenomenon of sizing is by far not a pure chemical process but rather a more physical one. Based on the gained findings it was possible so far to optimize the ASA sizing process in industrial-scale by means of ~ 50% less ASA consumption at a steady degree of sizing and improved physical sheet properties.
|
177 |
Stabil och antibiotikafri läkemedelsproduktion i rekombinant Escherichia coliBenevides, Kristina, Broström, Oscar, Elison Kalman, Grim, Swenson, Hugo, Vlassov, Andrei, Ågren, Josefin January 2017 (has links)
Den här rapporten presenterar ett antibiotikafritt, stabilt och kromosombaserat expressionssystem för läkemedelsproduktion i Escherichia coli på beställning av företaget Affibody AB. E. coli-stammen BL21(DE3) valdes som värdorganism för expressionssystemet. Systemet består av en genkassett som innehåller en T7-promotor, en 5′-UTR från genen ompA och en terminatorsekvens från RNA-operonet rrnB. Fyra kopior av genkassetten ska integreras i pseudogenerna caiB, yjjM, hsdS och yjiV. En datormodell som modellerar det egentliga kopietalet i cellerna har skapats i mjukvaran MATLAB, vilket visar att det uppskattas vara maximalt 32 kopior av genkassetten per cell på grund av replikation av kromosomen. Ett högt pH i fermentorn; att använda fed-batch och blandade kolhydratkällor; och att använda stammen BL21(DE3) minskar acetatproduktionen i cellen. En lägre acetatproduktion kan leda till en högre produkthalt. En proteinutbytesmodell för mjukvaran MATLAB har konstruerats för att uppskatta koncentrationen av Affibody®-molekylen i en E. coli cell.
|
178 |
Physico-Chemical Processes during Reactive Paper Sizing with Alkenyl Succinic Anhydride (ASA)Porkert, Sebastian 09 December 2016 (has links)
Sizing (hydrophobization) is one of the most important process steps within the added-value chain of about 1/3rd of the worldwide produced paper & board products. Even though sizing with so-called reactive sizing agents, such as alkenyl succinic anhydride (ASA) was implemented in the paper industry decades ago, there is no total clarity yet about the detailed chemical and physical mechanisms that lead to their performance. Previous research was carried out on the role of different factors influencing the sizing performance, such as bonding between ASA and cellulose, ASA hydrolysis, size revision as well as the most important interactions with stock components, process parameters and additives during the paper making process. However, it was not yet possible to develop a holistic model for the explanation of the sizing performance given in real life application. This thesis describes a novel physico-chemical approach to this problem by including results from previous research and combining these with a wide field of own basic research and a newly developed method that allows tracing back the actual localization of ASA within the sheet structure.
The carried out measurements and trial sets for the basic field of research served to evaluate the stock and process parameters that most dominantly influence the sizing performance of ASA. Interactions with additives other than retention aids were not taken into account. The results show that parameters, such as the content of secondary fibers, the degree of refining, the water hardness as well as the suspension conductivity, are of highest significance. The sample sets of the trials with the major impacting parameters were additionally analyzed by a newly developed localization method in order to better understand the main influencing factors.
This method is based on optical localization of ASA within the sheet structure by confocal white light microscopy. In order to fulfill the requirements at magnification rates of factor 100 optical zoom, it was necessary to improve the contrast between ASA and cellulose. Therefore, ASA was pretreated with an inert red diazo dye, which does not have any impact on neither the sizing nor the handling properties of ASA. Laboratory hand sheets that were sized with dyed ASA, were analyzed by means of their sizing performance in correlation to measurable ASA agglomerations in the sheet structure. The sizing performance was measured by ultrasonic penetration analysis. The agglomeration behavior of ASA was analyzed automatically by multiple random imaging of a sample area of approx. 8650 µm² with a minimum resolution for particles of 500 nm in size. The gained results were interpreted by full factorial design of experiments (DOE). The trials were carried out with ASA dosages between 0% and 0.8% on laboratory hand sheets, made of 80% bleached eucalyptus short fiber kraft pulp and 20% northern bleached softwood kraft pulp, beaten to SR° 30, produced with a RDA sheet former at a base weight of 100 g/m² oven dry.
The results show that there is a defined correlation between the ASA dosage, the sizing performance and the number and area of ASA agglomerates to be found in the sheet structure. It was also possible to show that the agglomeration behavior is highly influenced by external factors like furnish composition and process parameters. This enables a new approach to the explanation of sizing performance, by making it possible to not only examine the performance of the sizing agent, but to closely look at the predominant position where it is located in the sheet structure. These results lead to the explanation that the phenomenon of sizing is by far not a pure chemical process but rather a more physical one. Based on the gained findings it was possible so far to optimize the ASA sizing process in industrial-scale by means of ~ 50% less ASA consumption at a steady degree of sizing and improved physical sheet properties.:Acknowledgment I
Abstract III
Table of Content V
List of Illustrations XI
List of Tables XVI
List of Formulas XVII
List of Abbreviations XVIII
1 Introduction and Problem Description 1
1.1 Initial Situation 1
1.2 Objective 2
2 Theoretical Approach 3
2.1 The Modern Paper & Board Industry on the Example of Germany 3
2.1.1 Raw Materials for the Production of Paper & Board 5
2.2 The Sizing of Paper & Board 8
2.2.1 Introduction to Paper & Board Sizing 8
2.2.2 The Definition of Paper & Board Sizing 10
2.2.3 The Global Markets for Sized Paper & Board Products and Sizing Agents 11
2.2.4 Physical and Chemical Background to the Mechanisms of Surface-Wetting and Penetration 13
2.2.4.1 Surface Wetting 14
2.2.4.2 Liquid Penetration 15
2.2.5 Surface and Internal Sizing 17
2.2.6 Sizing Agents 18
2.2.6.1 Alkenyl Succinic Anhydride (ASA) 19
2.2.6.2 Rosin Sizes 19
2.2.6.3 Alkylketen Dimer (AKD) 23
2.2.6.4 Polymeric Sizing Agents (PSA) 26
2.2.7 Determination of the Sizing Degree (Performance Analysis) 28
2.2.7.1 Cobb Water Absorption 29
2.2.7.2 Contact Angle Measurement 30
2.2.7.3 Penetration Dynamics Analysis 31
2.2.7.4 Further Qualitative Analysis Methods 33
2.2.7.4.1 Ink Stroke 33
2.2.7.4.2 Immersion Test 33
2.2.7.4.3 Floating Test 34
2.2.7.4.4 Hercules Sizing Tester (HST) 34
2.2.8 Sizing Agent Detection (Qualitative Analysis) and Determination of the Sizing Agent Content (Quantitative Analysis) 35
2.2.8.1 Destructive Methods 35
2.2.8.2 Non Destructive Methods 36
2.3 Alkenyl Succinic Anhydride (ASA) 36
2.3.1.1 Chemical Composition and Production of ASA 37
2.3.1.2 Mechanistic Reaction Models 39
2.3.1.3 ASA Application 42
2.3.1.3.1 Emulsification 42
2.3.1.3.2 Dosing 44
2.3.1.4 Mechanistic Steps of ASA Sizing 46
2.3.2 Physico-Chemical Aspects during ASA Sizing 48
2.3.2.1 Reaction Plausibility 48
2.3.2.1.1 Educt-Product Balance / Kinetics 48
2.3.2.1.2 Energetics 51
2.3.2.1.3 Sterics 52
2.3.2.2 Phenomena based on Sizing Agent Mobility 53
2.3.2.2.1 Sizing Agent Orientation 54
2.3.2.2.2 Intra-Molecular Orientation 55
2.3.2.2.3 Sizing Agent Agglomeration 55
2.3.2.2.4 Fugitive Sizing / Sizing Loss / Size Reversion 56
2.3.2.2.5 Sizing Agent Migration 58
2.3.2.2.6 Sizing Reactivation / Sizing Agent Reorientation 59
2.3.3 Causes for Interactions during ASA Sizing 60
2.3.3.1 Process Parameters 61
2.3.3.1.1 Temperature 61
2.3.3.1.2 pH-Value 62
2.3.3.1.3 Water Hardness 63
2.3.3.2 Fiber Types 64
2.3.3.3 Filler Types 65
2.3.3.4 Cationic Additives 66
2.3.3.5 Anionic Additives 67
2.3.3.6 Surface-Active Additives 68
2.4 Limitations of State-of-the-Art ASA-Sizing Analysis 69
2.5 Optical ASA Localization 71
2.5.1 General Background 71
2.5.2 Confocal Microscopy 72
2.5.2.1 Principle 72
2.5.2.2 Features, Advantage and Applicability for Paper-Component Analysis 74
2.5.3 Dying / Staining 75
3 Discussion of Results 77
3.1 Localization of ASA within the Sheet Structure 77
3.1.1 Choice of Dyes 77
3.1.1.1 Dye Type 78
3.1.1.2 Evaluation of Dye/ASA Mixtures 80
3.1.1.2.1 Maximum Soluble Dye Concentration 80
3.1.1.2.2 Thin Layer Chromatography 81
3.1.1.2.3 FTIR-Spectroscopy 82
3.1.1.3 Evaluation of the D-ASA Emulsion 84
3.1.1.4 Paper Chromatography with D-ASA & F-ASA Emulsions 85
3.1.1.5 Evaluation of the D-ASA Emulsion’s Sizing Efficiency 86
3.1.2 The Localization Method 87
3.1.2.1 The Correlation between ASA Distribution and Agglomeration 88
3.1.2.2 Measurement Settings 89
3.1.2.3 Manual Analysis 90
3.1.2.4 Automated Analysis 92
3.1.2.4.1 Automated Localization / Microscopy Measurement 92
3.1.2.4.2 Automated Analysis / Image-Processing 93
3.1.2.5 Result Interpretation and Example Results 96
3.1.2.6 Reproducibility 97
3.1.2.7 Sample Mapping 98
3.1.3 Approaches to Localization-Method Validation 102
3.1.3.1 Raman Spectroscopy 102
3.1.3.2 Confocal Laser Scanning Fluorescent Microscopy 102
3.1.3.3 Decolorization 103
3.2 Factors Impacting the Sizing Behavior of ASA 104
3.2.1 ASA Type 105
3.2.2 Emulsion Parameters 107
3.2.2.1 Hydrolyzed ASA Content 107
3.2.2.2 ASA/Starch Ratio 109
3.2.2.3 Emulsion Age 110
3.2.3 Stock Parameters 111
3.2.3.1 Long Fiber/Short Fiber Ratio 111
3.2.3.2 Furnish Type 112
3.2.3.3 Degree of Refining 114
3.2.3.4 Filler Type/Content 116
3.2.4 Process Parameters 119
3.2.4.1 Temperature 119
3.2.4.2 pH-Value 120
3.2.4.3 Conductivity 122
3.2.4.4 Water Hardness 123
3.2.4.5 Shear Rate 125
3.2.4.6 Dwell Time 127
3.2.4.7 Dosing Position & Dosing Order 128
3.2.4.8 Drying 130
3.2.4.9 Aging 131
3.3 Factors Impacting the Localization Behavior of ASA 132
3.3.1 Degree of Refining 132
3.3.2 Sheet Forming Conductivity 135
3.3.3 Water Hardness 136
3.3.4 Retention Aid (PAM) 137
3.3.5 Contact Curing 138
3.3.6 Accelerated Aging 139
3.4 Main Optimization Approach 141
3.4.1 Optimization of ASA Sizing Performance Characteristics 142
3.4.2 Emulsion Modification 144
3.4.2.1 Lab Trials / RDA Sheet Forming 146
3.4.2.2 TPM Trials 147
3.4.2.3 Industrial-Scale Trials 149
3.4.2.4 Correlation between Sizing Performance Optimization and Agglomeration Behavior on the Example of PAAE 152
3.5 Holistic Approach to Sizing Performance Explanation 154
4 Experimental Approach 157
4.1 Characterization of Methods, Measurements and Chemicals used for the Optical Localization-Analysis of ASA 157
4.1.1 Characterization of used Chemicals 157
4.1.1.1 Preparation of Dyed-ASA Solutions 157
4.1.1.2 Thin Layer Chromatography 157
4.1.1.3 Fourier Transformed Infrared Spectroscopy 157
4.1.1.4 Emulsification of ASA 158
4.1.1.5 Paper Chromatography 159
4.1.1.6 Particle Size Measurement 159
4.1.2 Optical Analysis of ASA Agglomerates 160
4.1.2.1 Microscopy 160
4.1.2.2 Automated Analysis 163
4.1.2.2.1 Adobe Photoshop 163
4.1.2.2.2 Adobe Illustrator 164
4.1.2.3 Confocal Laser Scanning Fluorescent Microscopy 166
4.2 Characterization of Used Standard Methods and Measurements 166
4.2.1 Stock and Paper Properties 166
4.2.1.1 Stock pH, Conductivity and Temperature Measurement 166
4.2.1.2 Dry Content / Consistency Measurement 167
4.2.1.3 Drainability (Schopper-Riegler) Measurement 167
4.2.1.4 Base Weight Measurement 168
4.2.1.5 Ultrasonic Penetration Measurement 168
4.2.1.6 Contact Angle Measurement 169
4.2.1.1 Cobb Measurement 169
4.2.1.2 Air Permeability Measurements 170
4.2.1.3 Tensile Strength Measurements 170
4.2.2 Preparation of Sample Sheets 171
4.2.2.1 Stock Preparation 171
4.2.2.2 Laboratory Refining (Valley Beater) 171
4.2.2.3 RDA Sheet Forming 171
4.2.2.4 Additive Dosing 173
4.2.2.5 Contact Curing 174
4.2.2.6 Hot Air Curing 174
4.2.2.7 Sample Aging 174
4.2.2.8 Preparation of Hydrolyzed ASA 175
4.2.2.9 Trial Paper Machine 175
4.2.2.10 Industrial-Scale Board Machine 177
4.3 Characterization of used Materials 178
4.3.1 Fibers 178
4.3.1.1 Reference Stock System 178
4.3.1.2 OCC Fibers 179
4.3.1.3 DIP Fibers 179
4.3.2 Fillers 180
4.3.3 Chemical Additives 180
4.3.3.1 ASA 180
4.3.3.2 Starches 181
4.3.3.3 Retention Aids 181
4.3.3.4 Poly Aluminum Compounds 181
4.3.3.5 Wet Strength Resin 181
4.3.4 Characterization of used Additives 182
4.3.4.1 Solids Content 182
4.4 Description of Implemented Advanced Data Analysis- and Visualization Methods 183
4.4.1 Design of Experiments (DOE183
4.4.2 Contour Plots 184
4.4.3 Box-Whisker Graphs 185
5 Conclusion 186
6 Outlook for Further Work 191
7 Bibliography 192
Appendix 207
7.1 Localization Method Reproducibility 207
7.2 DOE - Coefficient Lists 208
7.2.1 Trial 3.3.4 – Impact of Retention Aid (PAM) on Agglomeration Behavior and Sizing Performance 208
7.2.2 Trial 3.3.5 – Impact of Contact Curing on Agglomeration Behavior and Sizing Performance 208
7.2.3 Trial 3.3.6 – Impact of Accelerated Aging on Agglomeration Behavior and Sizing Performance 209
|
179 |
Primary health care challenges in Ekurhuleni Metropolitan MunicipalityNdhambi, Mshoni Angeline 01 February 2013 (has links)
OBJECTIVE/ METHOD
The study examined implementation challenges faced by primary health care workers within the Ekurhuleni Metropolitan Municipality in Gauteng South Africa. Data collection was based on semi-structured interviews carried out on a purposive sample (n=19) of frontline clinicians working within the district as primary health care practitioners.
RESULTS
Participants confirmed that work within the primary health care service disproportionately focussed on curative and rehabilitative functions of their roles with little prioritisation of preventive and promotive interventions. Primary identified reasons included, institutional culture that prioritised short-term curative approaches. Clinicians also cited a range of other organisational barriers, such as – poor strategic planning, and a lack of understanding of health promotion and illness prevention.
CONCLUSIONS
Although the challenges that exist in implementing primary health care are clearly understood, clinicians perceive the solutions for these as being within the control of policy makers and those with power within the organisation. / Health Studies / M.A. (Public Health)
|
180 |
Thérapie génique ciblant CD33 dans les cellules souches hématopoïétiques, une approche innovatrice pour le traitement de la leucémie myéloïde aiguëTremblay-Laganière, Camille 09 1900 (has links)
No description available.
|
Page generated in 1.4108 seconds