Luminescence de l'argent dans les phosphates

Belharouak, Ilias

05 October 1999

Le but de ce travail était d'étudier et de caractériser la luminescence de l'argent dans les matériaux phosphatés, qu'ils soient cristallisés ou vitreux. Trois types de centres photoluminescents ont été mis en évidence : le premier centre, appelé (A) est caractéristique des transitions dans les phases AgM(PO3)3 (M = Mg, Zn, Ba) et Na2-xAgxZnP2O7 dont les structures ont été complètement déterminées. La dynamique de son émission peut être expliquée dans la plupart des cas par un système à trois niveaux. Le centre (C) est attribué à des "paires" d'argent. En effet, lorsque les structures cristallines le permettent, des interactions indirectes Ag+--Ag+ peuvent se développer entre deux cations voisins, chacun occupant son propre site cristallochimique. Un type particulier d'interaction d10--d10 a pu être rencontré, il s'agit des associations Ag+--Zn2+ dont l'existence est suggérée pour expliquer la présence de l'émission (C) détectée dans le polyphosphate AgZn(PO3)3. La fluorescence (B) est détectée à la périphérie des agrégats micrométriques d'argent métallique dans les verres phosphosilicate du système "P2O5-SiO2-ZnO-Ag2O". Ses caractéristiques spécifiques ont permis de l'associer à un type d'interaction différent, en l'occurence à des interactions Ag0--Ag+.

[CHIM:MATE] Chimie/Matériaux

Photoluminescence

Argent monovalent

Paries d'argent

Agrégats d'argent métallique

Polyphosphate

Diphosphate

Absorption X

Verres oxydes

Enhancing Interfacial Bonding of a Biodegradable Calcium Polyphosphate/Polyvinyl-urethane Carbonate Interpenetrating Phase Composite for Load Bearing Fracture Fixation Applications

Guo, Yi

06 April 2010

This thesis describe methods to improve the interfacial stability of an interpenetrating phase composite (IPC) polyvinylurethanecarbonate), and to increase the hydrophobicity of the polymer phase. The current IPCs introduce covalent bonding between the phases via silanizing agents to enhance the interfacial stability. Incorporation of the silanizing agents was also intended to reduce the IPC’s sensitivity to interfacial hydration, thereby enhancing the IPC’s resistance to degradation during aging. Lysine diisocyanate was used to increase the hydrophobic character in the polyvinylurethanecarbonate resin. The polymer resins were infiltrated into porous CPP blocks with 25 volume% interconnected porosity and polymerized to produce the IPCs. After mechanical testing following a aging study it was found that the silanizing agents contributed to stability of the mechanical properties under aqueous conditions. It was concluded that the mechanical properties and stability were comparable to available biodegradable composites, as well as being biocompatible to a preosteoblast model cell line.

Orthopaedic

Interpenetrating Phase Composite

Calcium Polyphosphate

Polyvinylurethane

Fracture Fixation

Load Bearing Bones

Biodegradable Composite

Mechanical Testing

silanizing agents

silane

0541

0794

Analysis and Quantification of Inositol Poly- and Pyrophosphates by NMR Spectroscopy and Mass Spectrometry

Puschmann, Robert

22 January 2020

Inositolpyrophosphate (PP-InsP) sind eine Gruppe sekundärer Signalmoleküle, die in einer Vielzahl zellulärer Prozesse, von Phosphathomeostase über Insulinsignalisierung bis Apoptose eine Rolle spielen. Die Art und Weise, wie PP-InsPs ihre Funktion ausführen, noch weitgehend unbekannt. Deshalb wurden zwei neue analytische Methoden basierend auf Kernspinresonanzspektroskopie und Flüssigchromatographie mit Massenspektrometrie-Kopplung (LCMS) entwickelt. Um die limitierende Sensitivität der Kernresonanzspektroskopie zu umgehen, wurde die Synthese von kernspinresonanzaktivem, 13C-markiertem Inositol optimiert. Des Weiteren wurde eine chemoenzymatische Synthese für alle Säugetier-PP-InsP-Isomere entwickelt, die auf der skalierbaren Ausfällung mittels Mg2+ Ionen basiert. Menschliche Zellen wurden mit 13C-Inositol isotopenmarkiert und in den Spektren der Zellextrakte wurde, basierend auf den PP-InsP-Standards, Fingerabdrucksignale identifiziert mit denen die Konzentrationen der dazugehörigen Moleküle bestimmt werden konnte. Die LCMS basierte Methode wurde auf dem Prinzip der Umsetzung von hochgeladenen Inositolpyrophosphaten zu ihren korrespondieren Methylestern mittels Trimethylsilyldiazomethan geplant. Die ungeladenen, permethylierten PP-InsPs wären geeignet für LC-Auftrennungen und MS-Messungen und sollten eine von Kernspinresonanzspektroskopie nicht erreichbare Sensitivität ermöglichen. Die Methode wurde mittels Inositolhexakisphosphat (InsP6), einem einfacheren PP-InsP-Analog, etabliert und methyliertes InsP6 konnte in Mengen von 10 femtomol detektiert werden. Die Adaption der Methode für die PP-InsPs gestaltete sich jedoch herausfordernd, da der Analyt während der Reaktion zersetzt wurde. Ein Wechsel zu Diazomethan als Methylierungsagens zeigte vielversprechende Resultate. / Inositol pyrophosphates (PP-InsPs) are a well conserved group of second messengers that are involved in a plethora of cellular processes including phosphate homeostasis, insulin signaling, and apoptosis. Despite much effort, it is still mostly unknown how PP-InsPs exert their diverse functions. In order to decipher the mechanisms, researchers have relied either on metabolic labeling with radioactive inositol or on electrophoretic separation on polyacrylamide gels but these methods either lack ease of use or sensitivity. Therefore, two new analytical tools, based on nuclear magnetic resonance (NMR) spectroscopy, and liquid chromatography coupled mass spectrometry (LCMS), were developed. To overcome the limited sensitivity provided by NMR spectroscopy, a high yielding synthesis of NMR-active 13C-labeled inositol was designed and optimized. Furthermore, a chemoenzymatic synthesis of all mammalian PP-InsPs isomers was developed that relied on a scalable purification strategy utilizing precipitation with Mg2+ ions. Human cells were metabolically labeled with 13C-inositol and the prepared PP-InsPs were used as standards to identify peaks in the NMRspectra. These fingerprint signals enabled the quantification of the corresponding molecules. The LCMS-based method was based on the derivatization of the highly charged inositol pyrophosphates to their corresponding methyl esters by trimethylsilyldiazomethane. The permethylated InsPs and PP-InsPs were suitable for LC separation and MS measurement, and provide a sensitivity unmatched by NMR spectroscopy. The method was established using inositol hexakisphosphate, a simpler analog of PP-InsPs, and methylated InsP6 could be detected at quantities as low as 10 femtomole. However, the adaptation of the derivatization for PP-InsPs proved challenging as the reaction caused degradation of the analyte but strategies to circumvent the decay by changing the derivatization agent to diazomethane were promising.

Inositolpyrophosphat

Inositolpolyphosphat

NMR Spektroskopie

Massenspektrometrie

Metabolomics

inositol polyphosphate

inositol pyrophosphate

NMR spectroscopy

Mass spectrometry

metabolomics

547 Organische Chemie

VK 8807

VG 9807

VG 9507

WD 5000

ddc:547

Elucidation of Inositol Polyphosphate Dephosphorylation Pathways using Stable-Isotope Labelling and NMR spectroscopy

Nguyen Trung, Minh

29 September 2023

Inositolpolyphosphate (InsPs) bilden eine ubiquitäre Gruppe an hochphosphorylierten, intrazellulären Signalmolekülen in eukaryotischen Zellen. Trotz deren Beteiligung an unzähligen biologischen Prozessen bleibt die Detektion von InsPs (insb. einzelner Enantiomere) eine Herausforderung, da die momentan verfügbaren Analysemethoden immer noch limitiert sind. In der vorliegenden Arbeit wird die stabile Isotopenmarkierung von myo-Inositol (Ins) und InsPs in Kombination mit Kernspinresonanzspektroskopie (engl. Nuclear Magnetic Resonance spectroscopy, NMR) erkundet, um diese Lücke zu schließen. Die Abhängigkeit von NMR-Daten und chemischer Struktur erlaubte die Analyse komplexer Mixturen aus InsPs aus in vitro-Experimenten und biologischen Proben. Durch stereospezifische 13C-Markierung konnten sogar Enantiomere voneinander unterschieden werden. Mit Hilfe dieser Methode wurden mehrere InsP-Stoffwechselwege untersucht. Als Erstes wurde das menschliche, Phytase-artige Enzym MINPP1 (engl. Multiple Inositol Polyphosphate Phosphatase 1) detailliert in vitro und in lebenden Zellen charakterisiert. Dabei wurde ein bisher unbeschriebener InsP-Stoffwechselweg in menschlichen Zellen erstmals beschrieben. Als Zweites wurden InsP verdauende Bakterien aus der menschlichen Darmflora untersucht, sodass der Abbauweg von Inositolhexakisphosphat beleuchtet werden konnte. Als Drittes wurden DUSP-Enzyme (engl. Dual-Specificity Phosphatases) identifiziert und in vitro charakterisiert, die in der Lage sind, die Phosphoanhydrid-Bindung von Inositolpyrophosphaten (PP-InsPs) zu spalten. Die vorliegende Arbeit demonstriert, dass 13C-Markierung in Verbindung mit NMR ein mächtiges Werkzeug darstellt, um InsP-Stoffwechselvorgänge zu untersuchen. / Inositol polyphosphates (InsPs) comprise a ubiquitous group of densely phosphorylated intracellular messengers in eukaryotic cells. Despite their contributions to a myriad of biological processes the detection of InsPs remains challenging to this day, especially with regards to differentiating enantiomers, as the available analytical toolset is still limited. In this thesis the use of stable isotope labelling of myo-inositol (Ins) and InsPs is explored to address this shortcoming. Combining 13C-labelling and nuclear magnetic resonance spectroscopy (NMR) provides both enhanced sensitivity and makes use of NMR’s strong structure-data dependency. This enabled the deconvolution of complex mixtures of InsPs from in vitro experiments or biological samples. With stereo-specific 13C-labels InsP mixtures could be resolved to individual enantiomers. Using this technique several InsP metabolic pathways were examined. Firstly, the human phytase-like enzyme Multiple Inositol Polyphosphate Phosphatase (MINPP1) was characterized in depth in vitro and in living cells, establishing a hitherto undescribed inositol polyphosphate metabolic path in humans. Secondly, inositol phosphate digesting bacteria isolated from the human gut microbiome were investigated, shedding light on the metabolic fate of inositol hexakisphosphate in the digestive track. Thirdly, a set of Dual-Specificity Phosphatases (DUSPs) were identified to be able to hydrolyze the phosphoanhydride bond of inositol pyrophosphates (PP-InsPs) and characterized in vitro. The 13C-labelling approach of InsPs in junction with NMR represents a powerful tool for the study of inositol polyphosphate metabolism. In the thesis at hand, this method has facilitated our understanding of inositol polyphosphate pathways and it will be continuing doing so in the future in several biological contexts.

myo-Inositolpolyphosphate

Inositolpyrophosphate

MINPP1

Phytase

Dephosphorylierung

NMR-Spektroskopie

Isotopen-Markierung

13C-Markierung

DUSP

intestinales Mikrobiom

kurzkettige Fettsäuren

Stoffwechselfluss-Analyse

Metabolitmarkierung

myo inositol polyphosphate

inositol pyrophosphate

MINPP1

phytase

dephosphorylation

NMR spectroscopy

isotope-label

13C-label

DUSP

dual-specificity phosphatase

gut microbiome

short-chain fatty acids

metabolic flux analysis

metabolic labelling

572 Biochemie

ddc:572

Análise do metabolismo de polifosfato e do operon pst em Pseudomonas aeruginosa. / Analysis of the metabolism of polyphosphate and of the pst operon in Pseudomonas aeruginosa.

Munevar, Nicolas Federico Villamil

06 August 2015

O operon pst de P. aeruginosa codifica um transportador de fosfato de alta afinida-de e também a proteína PhoU que, em conjunto, atuam como repressores da ex-pressão do regulon Pho dessa espécie. A atividade de PhoU está também associada ao metabolismo de polifosfato (poliP), dado que mutantes phoU nulos apresentam um vasto acúmulo do biopolímero. Ensaios de β-galactosidase mostraram uma alteração na expressão dos genes ppk e ppx, envolvidos no metabolismo de poliP, no mutante phoU. Observou-se que na cepa selvagem, a transcrição de ppk e de ppx não responde às limitações de Pi ou de nitrogênio, sendo esses genes altamente expressos em condições normais de crescimento. Além disso, determinou-se que ppk é co-transcrito com o gene hemB, os quais formam, portanto, um operon. O operon pst também foi analisado. Foi identificado por ensaios de northern blot o transcrito do primeiro gene do operon, pstS, que codifica uma proteína periplasmática. Também, foi identificado um promotor imediatamente a montante de phoU, o gene mais distal do operon, que permitiria sua expressão em condições normais do crescimento bacteriano. Por fim, determinou-se por ensaios de EMSA que as duas sequências consenso Pho box presentes no operon pst são completamente funcionais. / The pst operon in P. aeruginosa encodes a high-affinity phosphate transporter and the PhoU protein, which together act as repressors of Pho regulon of this species. The PhoU activity is also related with polyphosphate (polyP) metabolism, since phoU null mutants have a large accumulation of the biopolymer. β-galactosidase assays allowed to confirm a change in the expression of ppk and ppx genes, in-volved in PolyP metabolism, in the phoU mutant. It was also evidenced that in the wild type strain, the ppk and ppx transcription does not respond to Pi or nitrogen starvation, and that these genes are highly expressed under conditions of normal growth. In addition, it was determined that ppk is co-transcribed with hemB, a gene involved in the synthesis of porphyrins, and they constitute therefore an operon. The pst operon was also examined. Was identified by northern blot the transcript of the first gene in the operon, pstS, which encodes a periplasmic protein. Also, a promoter was identified immediately upstream of phoU, the most distal gene in the operon, allowing its expression in normal conditions of bacterial growth. Finally, it was determined by EMSA that the two consensus sequences Pho box present in the pst operon are fully functional.

phoU

phoU

ppk

ppk

ppx

ppx

Pseudomonas aeruginosa

Pseudomonas aeruginosa

pst operon

Fosfato

Gene regulation

Operon

Operon

Operon pst

Pho box

Pho box

Pho regulon

Polifosfato

Polyphosphate

Pst transporter

Regulação gênica

Regulon Pho

Transportador Pst

Análise do metabolismo de polifosfato e do operon pst em Pseudomonas aeruginosa. / Analysis of the metabolism of polyphosphate and of the pst operon in Pseudomonas aeruginosa.

Nicolas Federico Villamil Munevar

06 August 2015

O operon pst de P. aeruginosa codifica um transportador de fosfato de alta afinida-de e também a proteína PhoU que, em conjunto, atuam como repressores da ex-pressão do regulon Pho dessa espécie. A atividade de PhoU está também associada ao metabolismo de polifosfato (poliP), dado que mutantes phoU nulos apresentam um vasto acúmulo do biopolímero. Ensaios de β-galactosidase mostraram uma alteração na expressão dos genes ppk e ppx, envolvidos no metabolismo de poliP, no mutante phoU. Observou-se que na cepa selvagem, a transcrição de ppk e de ppx não responde às limitações de Pi ou de nitrogênio, sendo esses genes altamente expressos em condições normais de crescimento. Além disso, determinou-se que ppk é co-transcrito com o gene hemB, os quais formam, portanto, um operon. O operon pst também foi analisado. Foi identificado por ensaios de northern blot o transcrito do primeiro gene do operon, pstS, que codifica uma proteína periplasmática. Também, foi identificado um promotor imediatamente a montante de phoU, o gene mais distal do operon, que permitiria sua expressão em condições normais do crescimento bacteriano. Por fim, determinou-se por ensaios de EMSA que as duas sequências consenso Pho box presentes no operon pst são completamente funcionais. / The pst operon in P. aeruginosa encodes a high-affinity phosphate transporter and the PhoU protein, which together act as repressors of Pho regulon of this species. The PhoU activity is also related with polyphosphate (polyP) metabolism, since phoU null mutants have a large accumulation of the biopolymer. β-galactosidase assays allowed to confirm a change in the expression of ppk and ppx genes, in-volved in PolyP metabolism, in the phoU mutant. It was also evidenced that in the wild type strain, the ppk and ppx transcription does not respond to Pi or nitrogen starvation, and that these genes are highly expressed under conditions of normal growth. In addition, it was determined that ppk is co-transcribed with hemB, a gene involved in the synthesis of porphyrins, and they constitute therefore an operon. The pst operon was also examined. Was identified by northern blot the transcript of the first gene in the operon, pstS, which encodes a periplasmic protein. Also, a promoter was identified immediately upstream of phoU, the most distal gene in the operon, allowing its expression in normal conditions of bacterial growth. Finally, it was determined by EMSA that the two consensus sequences Pho box present in the pst operon are fully functional.

phoU

ppk

ppx

Pseudomonas aeruginosa

Fosfato

Operon

Operon pst

Pho box

Polifosfato

Regulação gênica

Regulon Pho

Transportador Pst

phoU

ppk

ppx

Pseudomonas aeruginosa

pst operon

Gene regulation

Operon

Pho box

Pho regulon

Polyphosphate

Pst transporter

New Analytical Tools to Interrogate Inositol Pyrophosphate Signaling

Harmel, Robert Klaus

26 June 2020

Inositolpyrophosphate (PP-InsPs) sind eine wichtige Gruppe eukaryotischer Botenstoffe, die mit verschiedenen Prozessen wie Apoptose, Phosphathomeostase und Insulinsignalkaskaden verknüpft sind. Trotz ihrer Entdeckung vor mehr als 20 Jahren bleibt es eine Herausforderung, die Signalmechanismen dieser Moleküle zu verstehen. Ursachen dafür sind der limitierte Zugang zu synthetischen PP-InsPs und ein Mangel an allgemein zugänglichen analytischen Methoden. Daher wurden in dieser Arbeit chemische und analytische Verfahren entwickelt, um unser Verständnis von diesen Molekülen sowohl auf ein biochemischer als auch auf zelluläre Ebene zu verbessern. Um der Knappheit an synthetischen PP-InsPs entgegen zu wirken, wurde eine hocheffiziente chemoenzymatische Synthese entwickelt, bei der mehr als 100 mg aller wesentlichen PP-InsPs aus Säugern hergestellt werden konnten. Parallel wurde ein neues analytisches Werkzeug entwickelt, dass Konzentrationen von PP-InsPs in komplexen Proben quantifizieren konnte. Mittels Enzymkatalyse konnten 13C-markiertes myo-inositol und 13C-markierte PP-InsPs hergestellt werden und niedrige Konzentrationen mit nuklearer Magnetresonanzspektroskopie detektiert werden. In vitro waren diese Verbindungen sehr nützlich, um PP-InsP Kinasen von Pflanzen und Säugern zu charakterisieren. Endogene Konzentrationen von PP-InsPs konnten durch metabolisches Markieren mit 13C-markiertem myo-inositol in humanen Zelllinien quantifiziert werden. Letztendlich wurde mittels eines neuen entwickelten proteomischen Ansatzes endogene Proteinpyrophosphorilierung, eine von PP-InsP eingebaute posttranslationale Proteinmodifikation, in menschlichen Zelllinien zum ersten Mal nachgewiesen. Zusammenfassend haben die aufgelisteten chemischen und analytischen Werkzeuge ein hohes Potenzial unser Verständnis der Signalmechanismen hinter den diversen Phänotypen der PP-InsPs zu stärken und Forschungsarbeit in dieser Richtung zu beschleunigen. / Inositol pyrophosphates (PP-InsPs) are an important group of second messengers that intersect with a wide range of processes in eukaryotic cells including phosphate homeostasis, insulin signaling and apoptosis. Despite their discovery more than two decades ago, elucidating the underlying signaling mechanisms remains a significant challenge. Therefore, a new set of chemical and analytical methods was developed here to improve our understanding of these intriguing molecules on the biochemical and cellular level. To overcome the shortage of synthetic PP-InsPs, a highly efficient and scalable chemoenzymatic approach was designed and the major mammalian PP-InsPs could be obtained in hundreds of milligram quantities and in high purity. In parallel, a new analytical tool was developed to quantify levels of PP-InsPs in complex samples. Chemoenzymatic access to 13C-labeled myo-inositol and 13C-labeled PP-InsPs enabled the detection of low concentrations of PP-InsPs using nuclear magnetic resonance spectroscopy. In vitro, these compounds were of great use for the biochemical characterization of PP-InsPs kinases from mammals and plants. Endogenous pools of PP-InsPs from human cell lines were identified and quantified by metabolic labeling with 13C-labeled myo-inositol. Finally, a new proteomics workflow towards the detection of protein pyrophosphorylation, a posttranslational modification mediated by PP-InsPs, using mass spectrometry was optimized and endogenously modified mammalian proteins could be identified for the first time and with high confidence. Taken together, the chemical and analytical tools presented here have great potential to accelerate the understanding of PP-InsP signaling and metabolism. Access to large amounts of PP-InsPs together with a reliable quantification method and the detection of endogenous protein pyrophosphorylation sites will be essential to unravel the signaling mechanisms underlying the diverse phenotypes associated with these metabolites.

Inositolpolyphosphat

Inositolpyrophosphat

NMR Spektroskopie

Proteomik

Massenspektrometrie

Metabolisches Markieren

Metabolomik

inositol polyphosphate

inositol pyrophosphate

NMR spectroscopy

proteomics

mass spectrometry

metabolic labeling

metabolomics

547 Organische Chemie

VK 8807

VG 9507

ddc:547

Identifying factors that correlate with Enhanced Biological Phosphorus Removal upsets at Lundåkraverket / Undersökning av faktorer som påverkar biologisk fosforavskiljning vid Lundåkraverket

Niranjan, Rounak

January 2021

The Enhanced Biological Phosphorus Removal (EBPR) process is characterized as the most sustainable process to remove phosphorus from wastewater albeit with high variability in performance efficiency. Thus, unpredictable upsets in the EBPR system is the norm across several wastewater treatment plants throughout Sweden, forcing the hand of the operators to dose higher volume of chemicals to reach the effluent requirements. As future effluent requirements are getting stricter and since higher chemical usage is environmentally and economically unsustainable, this investigation was setup to evaluate which environmental, operational and/or wastewater characteristics correlate with EBPR upsets at full-scale wastewater treatment plant (WWTP), more specifically at Lundåkra WWTP operated by Nordvästra Skånes Vatten och Avlopp (NSVA). The data used in the investigation was collected between 1St January 2018 and 31St December 2020 for a vast number of parameters known to play a key role in biological phosphorus removal. Online sensors as well as external and internal analysis contributed to the data which included parameters such as ‘Total flow at the plant’, ‘pH of the incoming water’, ‘Temperature in aeration basins’, ‘Dissolved oxygen (DO) levels in aeration basins’, ‘Nitrate in aeration basins’, ‘Sludge content in aeration basins’, etc. Other relevant parameters such as ‘Hydraulic retention time (HRT) in the treatment units’, ‘Sludge retention time (SRT) in aeration basin’, ‘Organic loading rate (OLR)’, etc. were calculated. Before the start of this investigation, the two possible explanations were presumed and they can be classified as: (i) upsets as a result of unsuitable environmental conditions and/or error in the operational strategy at the plant and (ii) upsets as a result of toxicity from higher concentration of metals in the influent specifically. Traditional statistical methods such as the t-distributed Stochastic Neighbor Embedding (t-SNE), Spearman Rank Correlation and Principal Component Analysis were used for the purpose of this study to test the first presumed explanation. The t-SNE plot showed that the upsets did not cluster into one large group but instead clamped up into smaller groups scattered across the length of the scale in both dimensions. This points towards the multivariate dependency of the EBPR process and exhibits that upsets might occur even with an operational strategy that produces good results otherwise. This, in turn, eludes to the fact that a non-included parameter such as the ‘daily metal concentrations in the influent’ could be responsible for some or all of the upsets. The Principal Component Analysis (PCA) plot, although noisy, offered an improvement strategy built around the key variables namely ‘nitrate in aeration basin 1 & 2’, ‘sludge content in aeration basin’, ‘SRT in aeration basin’, ‘O2 in aeration basin 1 & 2’ and ‘pH of incoming water’. Therefore, it is recommended that an improvement strategy be devised around them. Multiple causal factors increase the complexity of the analysis by decreasing the correlation coefficients, however, incorporation of the scatterplots presents a clearer picture. The parameters ‘nitrate in aeration basin 1 & 2’ and ‘sludge content in aeration basin’ showed the strongest correlation with phosphate values at the end of biological treatment at -0.32 and 0.42 respectively. The results also open the door to future research and provide direction for further investigations. / Den förbättrade biologiska fosforborttagningsprocessen karakteriseras som den mest hållbara processen för att avlägsna fosfor från avloppsvatten om än med stor variation i prestandaeffektivitet. Således är oförutsägbara störningar i systemet för förbättrad biologisk fosforavskiljning (EBPR) normen bland flera avloppsreningsverk i hela Sverige, vilket tvingar operatörerna att dosera högre volymer kemikalier för att nå avloppskraven. Eftersom framtida avloppskrav blir allt strängare och eftersom högre kemikalieanvändning är miljömässigt och ekonomiskt ohållbar, gjordes denna undersökning för att utvärdera vilka miljö-, drifts- och/eller avloppsvattenegenskaper som korrelerar med EBPR- störningar vid fullskaligt avloppsreningsverk. Närmare bestämt vid Lundåkra reningsverk som drivs av Nordvästra Skånes Vatten och Avlopp. Datan som användes i undersökningen samlades in mellan 1:a januari 2018 och 31:a december 2020 för ett fast antal parametrar som är kända att spela en nyckelroll vid borttagning av biologiskt P. Onlinesensorer samt externa och interna analyser bidrog till datan vilken inkluderade parametrar som 'Totalt flöde vid anläggningen', 'pH för det inkommande vattnet', 'Temperatur i luftningsbassänger', nivåer av upplöst syre (DO) i luftningsbassänger ',' Nitrat i luftningsbassänger ',' Slamhalt i luftningsbassänger ', etc. Andra relevanta parametrar som 'Hydraulisk retentionstid (HRT) i behandlingsenheterna ',' Slamretentionstid (SRT) i luftningsbassäng ',' Organisk belastningshastighet (OLR) ', etc. beräknades. Innan denna undersökning påbjörades antogs de två möjliga förklaringarna och de kan klassificeras som: (i) störningar till följd av olämpliga miljöförhållanden och/eller fel i driftstrategin vid anläggningen och (ii) störningar till följd av toxicitet från högre koncentration av metaller i inflödet specifikt. Traditionella statistiska metoder såsom t- Distributed Stochastic Neighbor Embedding (t-SNE), Spearman Rank Correlation och Principal Component Analysis användes i denna studie för att testa den första förmodade förklaringen. t-SNE- diagrammet visade att störningarna inte samlades i en stor grupp utan istället klämdes ihop i mindre grupper utspridda över skalans längd i båda dimensionerna. Detta pekar mot EBPR-processens multivariata beroende och visar att störningar kan uppstå även med en operativ strategi som annars ger bra resultat. Detta i sin tur undviker det faktum att en icke-inkluderad parameter som "dagliga metallkoncentrationer i inflödet" kan vara orsaken för några eller alla störningar. Principal Component Analysis (PCA)-diagrammet, trots att det var bullrigt, möjliggjorde en förbättringsstrategi byggd kring nyckelvariablerna, nämligen 'nitrat i luftningsbassäng 1 & 2', 'slamhalt i luftningsbassäng', 'SRT i luftningsbassäng', 'O2 i luftningsbassäng 1 & 2' och 'pH av inkommande vatten'. Därför rekommenderas att en förbättringsstrategi utarbetas kring dem. Flera kausala faktorer ökar komplexiteten i analysen genom att minska korrelationskoefficienterna, men spridningsdiagrammen ger en tydligare bild. Parametrarna ‘nitrat i luftningsbassäng 1 & 2’ och ‘slamhalt i luftningsbassäng’ visade starkast samband med fosfatvärden vid slutet av biologisk behandling vid -0,32 respektive 0,42. Resultaten lämnar dörren öppen för framtida forskning och kan vägleda vidare undersökningar.

Enhanced biological phosphorus removal

polyphosphate accumulating organisms

glycogen accumulating organisms

sludge content in aeration basin

nitrates in aeration basin

pH of incoming water

principal component analysis

pairwise correlations

inhibition factors

Engineering and Technology

Teknik och teknologier

Identifizierung und Charakterisierung exogener und endogener endothelialer Faktoren für die Ätiopathogenese der Atherosklerose

Tölle, Markus

31 May 2006

Für die Ätiopathogenese der Atherosklerose spielen eine Vielzahl von Mediatoren eine Rolle. Dabei werden durch das Endothel sowohl protektive als auch schädliche Mediatoren sezerniert. High Density Lipoproteine (HDL) stellen einen bedeutenden protektiven Marker für das kardiovaskuläre Risiko dar, u.a. durch die Aktivierung der endothelialen NO-Synthase (eNOS). HDL besteht zu 50 % aus Proteinen und zu 50 % aus Lipiden. Welche Komponenten des HDL für die eNOS Aktivierung verantwortlich sind, ist nicht bekannt gewesen. Im ersten Abschnitt dieser Promotionsarbeit konnte erfolgreich gezeigt werden, dass die Lysophospholipide, Sphingosin-1-Phosphat (S1P) und Sphinsosylphosphorylcholin (SPC), die strukturelle Bestandteile der Lipidfraktion von HDL darstellen, für einen Teil der HDL induzierten eNOS Aktivierung durch Stimulation des S1P3-Rezeptors verantwortlich sind. Diese eNOS Aktivierung wird durch den intrazellulären Einstrom von Calcium und durch die Aktivierung der Akt-Kinase induziert. Im zweiten Abschnitt dieser Promotionsarbeit konnte nachgewiesen werden, dass das oral verfügbare Lysophospholipid-basierte Medikament, FTY720, das ein strukturelles Analogon des S1P ist, den HDL induzierten Signaltransduktionsweg der eNOS Aktivierung in gleicher Weise induziert. Im dritten Abschnitt dieser Promotionsarbeit konnte ein neuartiges endothelabhängig sezerniertes gemischtes Dinukleosidpolyphosphat, Uridin-Adenosin-Tetraphosphat (Up4A), identifiziert werden. Up4A ist ein Agonist an den P2X- und P2Y-Purinrezeptoren. Up4A induziert bei Applikation in eine isoliert perfundierte Rattenniere hauptsächlich über die Aktivierung des P2X1-Rezeptors und des P2Y2/P2Y4-Rezeptors eine starke Vasokonstriktion im renalen Perfusionsgebiet mit einhergehender Erhöhung des mittleren renalen Perfusionsdrucks. Die direkte Infusion von Up4A in vivo in eine WKY-Ratte führt zu einer signifikanten Erhöhung des mittleren arteriellen Blutdrucks. / In the pathogenesis of atherosclerosis many mediators are included. Therefore the endothelium plays a crucial part by secreting protective but also deleterious factors. High density lipoproteins are an established protective factor in the risk profile of cardiovascular events especially by activating the endothelial NO synthase (eNOS). HDL is composed of 50 % proteins and 50 % lipids. Which component of HDL is responsible for the eNOS activation was not known. In the first part of this dissertation it could be shown, that the lysophospholipids, sphingosine-1-phosphate (S1P) and sphingosylphosphorylcholine (SPC), which are structural compounds of the lipid fraction of HDL, are responsible for a significant part of the HDL induced eNOS activation by stimulating the specific S1P3 receptor. In the signal transduction mechanism the activation of Akt kinase and an influx of calcium is involved. In the second part of this dissertation it could be shown, that the orally active lysophospholipide based drug FTY720, which is a structural analogue of S1P, is able to induce the same signal transduction mechanism activated by HDL including the stimulation of the S1P3 receptor. In the last part of this dissertation a new endothelium dependent vasoconstrictor, the dinucleoside polyphosphate uridine-adenosine-tetraphosphate (Up4A), could be for the first time identified. Up4A is a potent agonist of the P2X- and P2Y-purinoceptors. Via activating the P2X1 receptor and the P2Y2/P2Y4 receptor Up4A induce a strong vasoconstriction in the renal perfusion system in the model of the isolated perfused rat kidney with an adjacent increase of the mean perfusion pressure. By injection of Up4A in vivo in a Wistar Kyoto rat the mean arterial pressure also increase significantly.

Atherosklerose

endotheliale NO-Synthase

High Density Lipoprotein

Lysophospholipide

Sphingosin-1-Phosphat

Sphingosylphosphorylcholin

S1P3-Rezeptor

Dinukleosidpolyphosphat

Uridin-Adenosin-Tetraphosphat

P2X1-Rezeptor

P2Y2-Rezeptor

P2Y4-Rezeptor

atherosclerosis

endothelial NO synthase

High Density Lipoprotein

lysophospholipide

sphingosine-1-phosphate

sphingosylphosphorylcholine

S1P3 receptor

dinucleoside polyphosphate

uridine-adenosine-tetraphosphate

P2X1 receptor

P2Y2 receptor

P2Y4 receptor

610 Medizin

33 Medizin

YC 1104

YC 1118

ddc:610

An Analysis of Grain Corn Nutritional Supplements and Relative Maturity in Mississippi

Whittenton, Joseph Bryan

04 May 2018

A review of available corn relative maturity groups in Mississippi shows a limited range of maturity groups in use. Research focusing on expanding the range of maturity groups was conducted in MS in 2015 and 2016. Along with expanded maturity groups, treatments of fertilizer (10-34-0), foliar zinc, and a plant hormone blend were studied to shorten the growing season. Four site years in MS were studied to determine optimal plant maturity group and treatment for length of season. The results showed decreased yield of 0.09-0.15 Mg ha-1 (1.5-2.3 bu ac-1) for each day of decreasing relative maturity in three of four site years. The addition of starter fertilizer increased vegetative growth stage, plant height V5 and V7, SPAD values at V5, and significantly decreases days to tassel and silking reproductive growth stages but did not affect yield.

NDRE

LREI

SI

ENDVI

GNDVI

NDVI

plants per acre

vegetation indices

30000

density

leaf area index

kernel column

kernel row

weight

kernel

tassel

plant height

brooksville

verona

starkville

mississippi

hybrid

maturity

foliar

2016

2015

corn

yield

spad

spectral

starter fertilizer

10-34-0

polyphosphate

fertilizer

zinc

hormone

ascend

pioneer

dekalb

relative maturity