Model order reduction for nonlinear problems in circuit simulation

Electrical circuits usually contain nonlinear components. Hence we are interested in MOR methods that can be applied to a system of nonlinear Differential-Algebraic Equations (DAEs). In particular we consider the TPWL (Trajectory PieceWise Linear) and POD (Proper Orthogonal Decomposition) methods. While the first one fully exploits linearity, the last method needs modifications to become efficient in evaluation. We describe a particular technique based on Missing Point Estimatio

Model order reduction for nonlinear problems in circuit simulation

Electrical circuits usually contain nonlinear components. Hence we are interested in MOR methods that can be applied to a system of nonlinear Differential-Algebraic Equations (DAEs). In particular we consider the TPWL (Trajectory PieceWise Linear) and POD (Proper Orthogonal Decomposition) methods. While the first one fully exploits linearity, the last method needs modifications to become efficient in evaluation. We describe a particular technique based on Missing Point Estimatio

Scaling Down Large-Scale Thawing of Monoclonal Antibody Solutions: 3D Temperature Profiles, Changes in Concentration, and Density Gradients

PURPOSE Scale-down devices (SDD) are designed to simulate large-scale thawing of protein drug substance, but require only a fraction of the material. To evaluate the performance of a new SDD that aims to predict thawing in large-scale 2 L bottles, we characterised 3D temperature profiles and changes in concentration and density in comparison to 125~mL and 2 L bottles. Differences in diffusion between a monoclonal antibody (mAb) and histidine buffer after thawing were examined. METHODS Temperature profiles at six distinct positions were recorded with type T thermocouples. Size-exclusion chromatography allowed quantification of mAb and histidine. Polysorbate 80 was quantified using a fluorescent dye assay. In addition, the solution's density at different locations in bottles and the SDD was identified. RESULTS The temperature profiles in the SDD and the large-scale 2 L bottle during thawing were similar. Significant concentration gradients were detected in the 2 L bottle leading to marked density gradients. The SDD slightly overestimated the dilution in the top region and the maximum concentrations at the bottom. Fast diffusion resulted in rapid equilibration of histidine. CONCLUSION The innovative SDD allows a realistic characterisation and helps to understand thawing processes of mAb solutions in large-scale 2 L bottles. Only a fraction of material is needed to gain insights into the thawing behaviour that is associated with several possible detrimental limitations

Successful bone marrow transplantation in a patient with DNA ligase IV deficiency and bone marrow failure

BACKGROUND: DNA Ligase IV deficiency syndrome is a rare autosomal recessive disorder caused by hypomorphic mutations in the DNA ligase IV gene (LIG4). The clinical phenotype shows overlap with a number of other rare syndromes, including Seckel syndrome, Nijmegen breakage syndrome, and Fanconi anemia. Thus the clinical diagnosis is often delayed and established by exclusion. METHODS: We describe a patient with pre- and postnatal growth retardation and dysmorphic facial features in whom the diagnoses of Seckel-, Dubowitz-, and Nijmegen breakage syndrome were variably considered. Cellular radiosensitivity in the absence of clinical manifestations of Ataxia telangiectasia lead to the diagnosis of DNA ligase IV (LIG4) deficiency syndrome, confirmed by compound heterozygous mutations in the LIG4 gene. At age 11, after a six year history of progressive bone marrow failure and increasing transfusion dependency the patient was treated with matched sibling donor hematopoetic stem cell transplantation (HSCT) using a fludarabine-based conditioning regimen without irradiation. RESULTS: The post-transplantation course was uneventful with rapid engraftment leading to complete and stable chimerism. Now at age 16, the patient has gained weight and is in good clinical condition. CONCLUSION: HSCT using mild conditioning without irradiation qualifies as treatment of choice in LIG4-deficient patients who have a matched sibling donor

The James Webb Space Telescope Mission

Twenty-six years ago a small committee report, building on earlier studies, expounded a compelling and poetic vision for the future of astronomy, calling for an infrared-optimized space telescope with an aperture of at least $4m$. With the support of their governments in the US, Europe, and Canada, 20,000 people realized that vision as the $6.5m$ James Webb Space Telescope. A generation of astronomers will celebrate their accomplishments for the life of the mission, potentially as long as 20 years, and beyond. This report and the scientific discoveries that follow are extended thank-you notes to the 20,000 team members. The telescope is working perfectly, with much better image quality than expected. In this and accompanying papers, we give a brief history, describe the observatory, outline its objectives and current observing program, and discuss the inventions and people who made it possible. We cite detailed reports on the design and the measured performance on orbit.Comment: Accepted by PASP for the special issue on The James Webb Space Telescope Overview, 29 pages, 4 figure

Prenatal exclusion/confirmation of Fanconi Anemia via flowcytometry

Die Zellzyklusanalyse an kultivierten Fruchtwasserzellen zur pränatalen Diagnostik der Fanconi-Anämie ist nicht hinreichend zuverlässig und sollte aufgrund der teilweisen Verfälschung des Ergebnisses durch tetraploide Zellen und unzureichende Mitogenantwort sowie eventuell einen hohen Anteil nichtstimulierbarer Zellen (sog. noncycling fraction) stets mit einer weiteren Untersuchung an Nabelschnurblutzellen bestätigt werden. Durch eine Kombination von Amnionzelll- und NS-Blut- Untersuchung mit Hilfe der Durchflußzytometrie kann die Diagnose FA dann in der Mehrzahl der Fälle sicher ausgeschlossen oder bestätigt werden. Diese funktionelle Testung ist insbesondere für das Screening von Niedrig-Risiko-Schwangerschaften geeignet, bei denen eine pränatale Diagnostik auf Grund eines auffälligen Ultraschallbefundes bei sonst leerer Familienanamnese durchgeführt wird. Indirekte und direkte Gendiagnostik setzen die Kenntnis des betroffenen Gens bzw. beider krankheitsverursachender Mutationen voraus. Im engen zeitlichen Fenster der pränatalen Diagnostik können diese nicht immer rechtzeitig bestimmt werden. In den Fällen, in welchen sowohl funktionelle als auch Gendiagnostik durchgeführt wurde, konnte das Ergebnis der funktionellen Diagnostik stets bestätigt werden. Die einzige Fehldiagnose unter den hier vorgestellten Familien beruhte auf der Tatsache, dass in diesem Fall das Ergebnis der Zellzyklustestung an kultivierten Fruchtwasserzellen nicht durch eine Untersuchung von Nabelschnurblut kontrolliert wurde. Werden sowohl Amnionzellen als auch Nabelschnurblut untersucht und wird die Untersuchung der Amnionzellen durch eine einfache Sensitivitätsmessung gegenüber MMC ergänzt, so ist die funktionelle pränatale Diagnostik eine verlässliche Methode zur Bestätigung oder zum Ausschluß der Diagnose Fanconi-Anämie. Die größtmögliche Sicherheit der pränatalen Diagnostik wird jedoch mit molekulargenetischen Methoden erreicht. Dies ist insbesondere dann der Fall, wenn Komplementationsgruppenzugehörigkeit und die Art der krankheitsverursachenden Mutationen vor Beginn der Schwangerschaft bekannt sind.Objective: To explore the potential of flowcytometry in the prenatal exclusion or confirmation of Fanconi anemia (FA). Methods: Indications for prenatal diagnosis were (1) FA-negative family history, but suspicious ultrasound findings such as radial ray aplasia, (2) FA-positive family history, but without knowledge of the affected gene and/or mutation. Amniotic fluid (AF) cell cultures and umbilical cord (UC) blood cultures were assayed for typical cell cycle changes (G2-phase accumulations) without and with Mitomycin C-treatments using single and dual parameter (BrdU-Hoechst) flowcytometry. Results: Single parameter flowcytometry correctly identified 2 positive and 9 negative cases on the basis of MMC-sensitivity of cultivated AF cells. Likewise, 8 negative cases and 2 positive cases were correctly predicted using bivariate flowcytometry of 72 h umbilical cord blood cultures. In contrast, bivariate flowcytometry applied to AF cells grown in the presence of bromodesoxyuridine (BrdU) yielded false positive and false negative results. Conclusions: Single parameter flowcytometry of AF-cell cultures and bivariate flowcytometry of UC-cell cultures have the potential to correctly predict the affected status in cases at risk for FA, whereas bivariate flow cytometry proved unreliable when applied to BrdU-substituted AF-cell cultures. Cases with a low a priori risk (e.g. sonographic finding of radial ray abnormalities and negative family history) would benefit most from flowcytometry as a rapid and economical prenatal screening procedure

Raman marker bands for secondary structure changes of frozen therapeutic monoclonal antibody formulations during thawing

In this work we use Raman spectroscopy for protein characterization in the frozen state. We investigate the behavior of frozen therapeutic monoclonal antibody IgG1 formulation upon thawing by Raman spectroscopy. Secondary and tertiary structure of the protein in three different mab formulations in the frozen state are followed through observation of marker bands for α-helix, β-sheet and random coil. We identify the tyrosine intensity ratio I856/I830 as a marker for mab aggregation. Upon fast cooling (40°C/min) to –80°C we observe a significant increase of random coil and α –helical structures, while this is not the case for slower cooling (20°C/min) to –80°C. Most changes in the protein's secondary structure are observed in the course of thawing in the range up to -20°C, when passing through the glass transitions and cold-crystallization of the two types of freeze-concentrated solutions formed through macro- and microcryoconcentration. An increase of protein concentration and the addition of mannitol suppress secondary structural changes but do no impact on aggregation

Data to the manuscript 'Imperfect cross-linking of Xanthan for pH-responsive bio-based composite moist wound dressings by stencil printing'

Evaluation data for the manuscript stated above. For follow-up evaluation, files have to be arranged according to file designation in the scripts uploaded. There is no additional description of how to arrange. Please feel free to contact the first author for help and information.Financial support is gratefully acknowledged to the COMET project "Textile Competence Center Vorarlberg 2 – FFG 882502" funded within COMET – Competence Centers for Excellent Technologies – by BMK, BMDW as well as co-financing federal province Vorarlberg. The COMET-Funding Program is managed by the Austrian Research Promotion Agency FFG. We also gratefully acknowledge funding by the Science Department of the State of Vorarlberg

Scaling Down Large-Scale Thawing of Monoclonal Antibody Solutions: 3D Temperature Profiles, Changes in Concentration, and Density Gradients.

Scale-down devices (SDD) are designed to simulate large-scale thawing of protein drug substance, but require only a fraction of the material. To evaluate the performance of a new SDD that aims to predict thawing in large-scale 2 L bottles, we characterised 3D temperature profiles and changes in concentration and density in comparison to 125 mL and 2 L bottles. Differences in diffusion between a monoclonal antibody (mAb) and histidine buffer after thawing were examined.Temperature profiles at six distinct positions were recorded with type T thermocouples. Size-exclusion chromatography allowed quantification of mAb and histidine. Polysorbate 80 was quantified using a fluorescent dye assay. In addition, the solution's density at different locations in bottles and the SDD was identified.The temperature profiles in the SDD and the large-scale 2 L bottle during thawing were similar. Significant concentration gradients were detected in the 2 L bottle leading to marked density gradients. The SDD slightly overestimated the dilution in the top region and the maximum concentrations at the bottom. Fast diffusion resulted in rapid equilibration of histidine.The innovative SDD allows a realistic characterisation and helps to understand thawing processes of mAb solutions in large-scale 2 L bottles. Only a fraction of material is needed to gain insights into the thawing behaviour that is associated with several possible detrimental limitations