Phytoplankton Communities in Temperate Rivers

Contant, Jacinthe

23 January 2012

The structure of phytoplankton communities was examined seasonally across five rivers with a focus on small cells and their relative importance. Picophytoplankton (0.2-2 μm), previously considered insignificant in rivers, reached densities as high as those observed in lakes and oceans (~ 10e4-10e5 cells/mL). Their relative importance was not a function of trophic state with the highest contribution to algal biomass found in the most eutrophic river. Body size distributions were analyzed from both chlorophyll-a size fractions and taxonomic enumerations; no significant effect of river or season was detected, suggesting that phytoplankton size distribution is not a useful metric of change in rivers. Unlike lake ecosystems, the rivers were uniformly dominated by small cells (< 20 μm). Taxonomic analyses of the seasonal succession did not reveal a common periodicity of particular divisions (e.g. diatoms). However, strong dominance was more typical of eutrophic rivers even though taxa richness was similar.

phytoplankton

picophytoplankton

size distribution analysis

seasonal succession

nutrients

Picophytoplankton in rivers

Phytoplankton Communities in Temperate Rivers

Contant, Jacinthe

23 January 2012

The structure of phytoplankton communities was examined seasonally across five rivers with a focus on small cells and their relative importance. Picophytoplankton (0.2-2 μm), previously considered insignificant in rivers, reached densities as high as those observed in lakes and oceans (~ 10e4-10e5 cells/mL). Their relative importance was not a function of trophic state with the highest contribution to algal biomass found in the most eutrophic river. Body size distributions were analyzed from both chlorophyll-a size fractions and taxonomic enumerations; no significant effect of river or season was detected, suggesting that phytoplankton size distribution is not a useful metric of change in rivers. Unlike lake ecosystems, the rivers were uniformly dominated by small cells (< 20 μm). Taxonomic analyses of the seasonal succession did not reveal a common periodicity of particular divisions (e.g. diatoms). However, strong dominance was more typical of eutrophic rivers even though taxa richness was similar.

phytoplankton

picophytoplankton

size distribution analysis

seasonal succession

nutrients

Picophytoplankton in rivers

Phytoplankton Communities in Temperate Rivers

Contant, Jacinthe

January 2012

The structure of phytoplankton communities was examined seasonally across five rivers with a focus on small cells and their relative importance. Picophytoplankton (0.2-2 μm), previously considered insignificant in rivers, reached densities as high as those observed in lakes and oceans (~ 10e4-10e5 cells/mL). Their relative importance was not a function of trophic state with the highest contribution to algal biomass found in the most eutrophic river. Body size distributions were analyzed from both chlorophyll-a size fractions and taxonomic enumerations; no significant effect of river or season was detected, suggesting that phytoplankton size distribution is not a useful metric of change in rivers. Unlike lake ecosystems, the rivers were uniformly dominated by small cells (< 20 μm). Taxonomic analyses of the seasonal succession did not reveal a common periodicity of particular divisions (e.g. diatoms). However, strong dominance was more typical of eutrophic rivers even though taxa richness was similar.

phytoplankton

picophytoplankton

size distribution analysis

seasonal succession

nutrients

Picophytoplankton in rivers

Forget the Weights, Who gets the Benefits? How to Bring a Poverty Focus to the Economic Analysis of Projects

Potts, David J.

06 1900

No / This paper examines the way in which the distributional impact of projects has been treated in the cost±bene®t analysis literature. It is suggested that excessive emphasis has been given to the estimation of distribution weights in the context of single ®gure measures of project worth and that more attention should be paid to estimation of the distribution e ects themselves. If projects really are to have some impact on poverty it is important that some attempt is made to measure what that impact is. Such an attempt requires both systematic measurement of direct income e ects as well as the possibility of measuring indirect e ects where these are expected to be important. An approach is suggested in which direct measurement of income e ects can be adjusted using shadow price estimates to determine indirect income e ects. The approach is illustrated with the example of a district heating project in the Republic of Latvia.

An automated multicolour fluorescence in situ hybridization workstation for the identification of clonally related cells

Dubrowski, Piotr

05 1900

The methods presented in this study are aimed at the identification of subpopulations (clones) of genetically similar cells within tissue samples through measurement of loci-specific Fluorescence in-situ hybridization (FISH) spot signals for each nucleus and analyzing cell spatial distributions by way of Voronoi tessellation and Delaunay triangulation to robustly define cell neighbourhoods. The motivation for the system is to examine lung cancer patient for subpopulations of Non-Small Cell Lung Cancer (NSCLC) cells with biologically meaningful gene copy-number profiles: patterns of genetic alterations statistically associated with resistance to cis-platinum/vinorelbine doublet chemotherapy treatment. Current technologies for gene-copy number profiling rely on large amount of cellular material, which is not always available and suffers from limited sensitivity to only the most dominant clone in often heterogeneous samples. Thus, through the use of FISH, the detection of gene copy-numbers is possible in unprocessed tissues, allowing identification of specific tumour clones with biologically relevant patterns of genetic aberrations. The tissue-wide characterization of multiplexed loci-specific FISH signals, described herein, is achieved through a fully automated, multicolour fluorescence imaging microscope and object segmentation algorithms to identify cell nuclei and FISH spots within. Related tumour clones are identified through analysis of robustly defined cell neighbourhoods and cell-to-cell connections for regions of cells with homogenous and highly interconnected FISH spot signal characteristics. This study presents experiments which demonstrate the system’s ability to accurately quantify FISH spot signals in various tumour tissues and in up to 5 colours simultaneously or more through multiple rounds of FISH staining. Furthermore, the system’s FISH-based cell classification performance is evaluated at a sensitivity of 84% and specificity 81% and clonal identification algorithm results are determined to be comparable to clone delineation by a human-observer. Additionally, guidelines and procedures to perform anticipated, routine analysis experiments are established.

Fluorescent in-situ hybridization

Tumour clones

Cancer genetics

Automated imaging

Spatial distribution analysis

Voronoi tessellation

Delaunay triangulation

Geoarchaelogical Investigation Of Central Anatolian Caravanserais Using Gis

Ertepinar Kaymakci, Pinar

01 June 2005

This study comprises analysis of geological, geomorphological constraints that played role in the site selection of caravanserais. In order to do this, 15 caravanserais located along a route from NevSehir-Aksaray-Konya to BeySehir were used. The data used in the study include a caravanserai database, lithological maps, and digital elevation model of the area. GIS analyses performed in the study are proximity, visibility, and probability distribution (PDA). The first step is the generation of the ancient trade route which is used as a reference in other analysis. Results of the analysis indicate that the average distance between consequent caravanserais is 10 km. PDA suggests that there should be two more caravanserais between BeySehir - Yunuslar and one caravanserai between Obruk - Sulatnahani hans. Caravanserais are very close to a water source but not at their immediate vicinity. Groundwater is not considered in this study / dominant water sources are streams, springs and lakes. Their visibility tested in an area of 78 km2 shows a great variation suggesting that visibility is not considered during the site selection. Ignimbrite, limestone and marble are preferred rocks types although other rocks such as clastic rocks are exposed in closer distances.

QE Geology 1-996.5

An automated multicolour fluorescence in situ hybridization workstation for the identification of clonally related cells

Dubrowski, Piotr

05 1900

The methods presented in this study are aimed at the identification of subpopulations (clones) of genetically similar cells within tissue samples through measurement of loci-specific Fluorescence in-situ hybridization (FISH) spot signals for each nucleus and analyzing cell spatial distributions by way of Voronoi tessellation and Delaunay triangulation to robustly define cell neighbourhoods. The motivation for the system is to examine lung cancer patient for subpopulations of Non-Small Cell Lung Cancer (NSCLC) cells with biologically meaningful gene copy-number profiles: patterns of genetic alterations statistically associated with resistance to cis-platinum/vinorelbine doublet chemotherapy treatment. Current technologies for gene-copy number profiling rely on large amount of cellular material, which is not always available and suffers from limited sensitivity to only the most dominant clone in often heterogeneous samples. Thus, through the use of FISH, the detection of gene copy-numbers is possible in unprocessed tissues, allowing identification of specific tumour clones with biologically relevant patterns of genetic aberrations. The tissue-wide characterization of multiplexed loci-specific FISH signals, described herein, is achieved through a fully automated, multicolour fluorescence imaging microscope and object segmentation algorithms to identify cell nuclei and FISH spots within. Related tumour clones are identified through analysis of robustly defined cell neighbourhoods and cell-to-cell connections for regions of cells with homogenous and highly interconnected FISH spot signal characteristics. This study presents experiments which demonstrate the system’s ability to accurately quantify FISH spot signals in various tumour tissues and in up to 5 colours simultaneously or more through multiple rounds of FISH staining. Furthermore, the system’s FISH-based cell classification performance is evaluated at a sensitivity of 84% and specificity 81% and clonal identification algorithm results are determined to be comparable to clone delineation by a human-observer. Additionally, guidelines and procedures to perform anticipated, routine analysis experiments are established.

Fluorescent in-situ hybridization

Tumour clones

Cancer genetics

Automated imaging

Spatial distribution analysis

Voronoi tessellation

Delaunay triangulation

An automated multicolour fluorescence in situ hybridization workstation for the identification of clonally related cells

Dubrowski, Piotr

05 1900

The methods presented in this study are aimed at the identification of subpopulations (clones) of genetically similar cells within tissue samples through measurement of loci-specific Fluorescence in-situ hybridization (FISH) spot signals for each nucleus and analyzing cell spatial distributions by way of Voronoi tessellation and Delaunay triangulation to robustly define cell neighbourhoods. The motivation for the system is to examine lung cancer patient for subpopulations of Non-Small Cell Lung Cancer (NSCLC) cells with biologically meaningful gene copy-number profiles: patterns of genetic alterations statistically associated with resistance to cis-platinum/vinorelbine doublet chemotherapy treatment. Current technologies for gene-copy number profiling rely on large amount of cellular material, which is not always available and suffers from limited sensitivity to only the most dominant clone in often heterogeneous samples. Thus, through the use of FISH, the detection of gene copy-numbers is possible in unprocessed tissues, allowing identification of specific tumour clones with biologically relevant patterns of genetic aberrations. The tissue-wide characterization of multiplexed loci-specific FISH signals, described herein, is achieved through a fully automated, multicolour fluorescence imaging microscope and object segmentation algorithms to identify cell nuclei and FISH spots within. Related tumour clones are identified through analysis of robustly defined cell neighbourhoods and cell-to-cell connections for regions of cells with homogenous and highly interconnected FISH spot signal characteristics. This study presents experiments which demonstrate the system’s ability to accurately quantify FISH spot signals in various tumour tissues and in up to 5 colours simultaneously or more through multiple rounds of FISH staining. Furthermore, the system’s FISH-based cell classification performance is evaluated at a sensitivity of 84% and specificity 81% and clonal identification algorithm results are determined to be comparable to clone delineation by a human-observer. Additionally, guidelines and procedures to perform anticipated, routine analysis experiments are established. / Science, Faculty of / Physics and Astronomy, Department of / Graduate

Fluorescent in-situ hybridization

Tumour clones

Cancer genetics

Automated imaging

Spatial distribution analysis

Voronoi tessellation

Delaunay triangulation

Infrared Imaging Decision Aid Tools for Diagnosis of Necrotizing Enterocolitis

Shi, Yangyu

09 July 2020

Neonatal necrotizing enterocolitis (NEC) is one of the most severe digestive tract emergencies in neonates, involving bowel edema, hemorrhage, and necrosis, and can lead to serious complications including death. Since it is difficult to diagnose early, the morbidity and mortality rates are high due to severe complications in later stages of NEC and thus early detection is key to the treatment of NEC. In this thesis, a novel automatic image acquisition and analysis system combining a color and depth (RGB-D) sensor with an infrared (IR) camera is proposed for NEC diagnosis. A design for sensors configuration and a data acquisition process are introduced. A calibration method between the three cameras is described which aims to ensure frames synchronization and observation consistency among the color, depth, and IR images. Subsequently, complete segmentation procedures based on the original color, depth, and IR information are proposed to automatically separate the human body from the background, remove other interfering items, identify feature points on the human body joints, distinguish the human torso and limbs, and extract the abdominal region of interest. Finally, first-order statistical analysis is performed on thermal data collected over the entire extracted abdominal region to compare differences in thermal data distribution between different patient groups. Experimental validation in a real clinical environment is reported and shows encouraging results.

NEC detection

infrared thermal imaging

RGB-D sensing

thermal distribution analysis

image processing

Scaling Relations as Cognitive Dipsticks: Distribution Analysis of Contextually Driven Performance Shifts in Three Linguistic Tasks

Annand, Colin T.

January 2017

No description available.

Cognitive Therapy

Cognitive Performance

Naming

Lexical Decision

Distribution Analysis

Word Recognition

Scaling