Antiserum titer determination and adherence comparison of three major outer membrane proteins TSA56, TSA47 and TSA22 in Orientia tsutsugamushi

Lin, Tung-cheng

07 September 2011

Orientia tsutsugamushi, the causative agent of scrub typhus, is an obligate intracellular pathogen. Recent studies show that the complete genome sequence of Orientia tsutsugamushi have been determined. However, the early signaling events involved in the entry of O.tsutsugamushi into mammalian cells remains a challenge. In this study, we demonstrate that adherence ability and comparison of three major outer membrane protein TSA56, TSA47 and TSA22 of O.tsutsugamushi. Through expression and purification of three type-specific antigen 56-kDa (include TSA56-antigen domain I, TSA56-antigen domain III), 47-kDa and 22-kDa of O. tsutsugamushi , antiserum immunoblots from 22 clinical O. tsutsugamushi-infected patients and in vitro adhesion assay of E.coli overexpression outer membrane protein of O. tsutsugamushi , the antiserum titer and adherence ability of bacterial outer membrane proteins are determined. The data show that antiserum titer against three major outer membrane proteins of O. tsutsugamushi was markedly higher in TSA56 compared to TSA47 and TSA22. In adhesion assay, adhesion of host cells by TSA56 was readily than TSA47 and TSA22. Furthermore, adhesion experiment and antiserum titer against antigen-domain I (ADI) region (19-114 aa) in the extracellular domain of TSA56 was also significantly higher than previously reported antigen-domain III(ADIII) region (237-366 aa) which facilitates the invasion of O. tsutsugamushi through interaction with fibronectin .Taken together, these results clearly indicate that O. tsutsugamushi exploits TSA56-mediated bacterial adhesion, abundant antiserum titer and ADI region of TSA56 may draw another adhesion site (except for previously reported ADIII) to invade eukaryotic host cells.

antiserum immunoblots

outer membrane protein

type-specific antigen

Orientia tsutsugamushi

scrub typhus

adhesion assay

ABVIC: A NOVEL FLOW CYTOMETRY-BASED ASSAY FOR THE DETECTION OF HSV-SPECIFIC ANTIBODIES

Sowa, Gavin Michael

01 December 2016

Herpes simplex virus type 1 (HSV-1) and herpes simplex virus type 2 (HSV-2) are closely related viruses that establish lifelong infection in their hosts and can periodically reactivate to cause painful lesions. Approximately 50 million Americans are infected with HSV-2, the primary cause of genital ulcerative disease. In addition to the pain of the physical symptoms, genital herpes is highly stigmatized and can cause significant reductions in quality of life. HSV-2 has been demonstrated to have a synergistic relationship with HIV, where it enhances the transmissibility, susceptibility and severity of disease. In addition, potentially life-threatening neonatal herpes occurs in about 1 in 10,000 live births. While there are known means of reducing the risk of transmission, the overwhelming majority of infected persons are unaware of their status, and they remain the driving force behind new infections. Virological tests, such as PCR, are ill suited for asymptomatic infections since the detectable virus is only shed on <10% of days. Currently available type-specific serological tests based on glycoprotein G are prone to false-positive results, lack the sensitivity to detect new infections and may be affected by cross-reactivity between HSV-1 and HSV-2. Due to the known limitations of HSV serological testing, it is not recommended for the general population or pregnant women. In the first half of my thesis, I evaluate a new flow-cytometry-based method that measures serum antibody-binding to virus-infected cells (ABVIC). We obtained a panel of human control sera from Westover Heights Clinic (WHC) and determined if the ABVIC could measure HSV-specific antibody binding to test-cells. We found that the assay was sensitive, semi-quantitative, and could be made type-specific with the addition of a pre-adsorption step. The ABVIC offers an advantage over the standard of care single-antigen tests as the result measuring antibody binding to all viral proteins fixed in their native conformation. In the second half of my thesis, I used the ABVIC assay test n=34 blinded test-sera. Of these, n=17 had previously tested as “indeterminate” by bother Herpeselect ELISA as well as Western Blot. Following unblinding, we found that the ABVIC properly identified all n=17 patient sera of an unambiguous serostatus. Of the indeterminate sera, all were found to be seronegative for HSV-2. Based on these surprising results, we requested an additional n=11 indeterminate samples, which were also found to be HSV-2 seronegative. Most of the "Indeterminate" serum samples exhibited high background, which produced weak reactivity in HerpeSelect and Western blot assays, but did not confound the internally controlled ABVIC test.

ABVIC

Diagnostics

Flow Cytometry

Herpes Simplex Virus

Serological testing

type-specific

Elucidation of Transcriptional Regulatory Mechanisms from Single-cell RNA-Sequencing Data

Ma, Anjun

January 2020

No description available.

Bioinformatics

Mathematical Expression Detection and Segmentation in Document Images

Bruce, Jacob Robert

19 March 2014

Various document layout analysis techniques are employed in order to enhance the accuracy of optical character recognition (OCR) in document images. Type-specific document layout analysis involves localizing and segmenting specific zones in an image so that they may be recognized by specialized OCR modules. Zones of interest include titles, headers/footers, paragraphs, images, mathematical expressions, chemical equations, musical notations, tables, circuit diagrams, among others. False positive/negative detections, oversegmentations, and undersegmentations made during the detection and segmentation stage will confuse a specialized OCR system and thus may result in garbled, incoherent output. In this work a mathematical expression detection and segmentation (MEDS) module is implemented and then thoroughly evaluated. The module is fully integrated with the open source OCR software, Tesseract, and is designed to function as a component of it. Evaluation is carried out on freely available public domain images so that future and existing techniques may be objectively compared. / Master of Science

document layout analysis

optical character recognition

document image

type-specific layout analysis

Development and encoding of visual statistics in the primary visual cortex

Rudiger, Philipp John Frederic

January 2017

How do circuits in the mammalian cerebral cortex encode properties of the sensory environment in a way that can drive adaptive behavior? This question is fundamental to neuroscience, but it has been very difficult to approach directly. Various computational and theoretical models can explain a wide range of phenomena observed in the primary visual cortex (V1), including the anatomical organization of its circuits, the development of functional properties like orientation tuning, and behavioral effects like surround modulation. However, so far no model has been able to bridge these levels of description to explain how the machinery that develops directly affects behavior. Bridging these levels is important, because phenomena at any one specific level can have many possible explanations, but there are far fewer possibilities to consider once all of the available evidence is taken into account. In this thesis we integrate the information gleaned about cortical development, circuit and cell-type specific interactions, and anatomical, behavioral and electrophysiological measurements, to develop a computational model of V1 that is constrained enough to make predictions across multiple levels of description. Through a series of models incorporating increasing levels of biophysical detail and becoming increasingly better constrained, we are able to make detailed predictions for the types of mechanistic interactions required for robust development of cortical maps that have a realistic anatomical organization, and thereby gain insight into the computations performed by the primary visual cortex. The initial models focus on how existing anatomical and electrophysiological knowledge can be integrated into previously abstract models to give a well-grounded and highly constrained account of the emergence of pattern-specific tuning in the primary visual cortex. More detailed models then address the interactions between specific excitatory and inhibitory cell classes in V1, and what role each cell type may play during development and function. Finally, we demonstrate how these cell classes come together to form a circuit that gives rise not only to robust development but also the development of realistic lateral connectivity patterns. Crucially, these patterns reflect the statistics of the visual environment to which the model was exposed during development. This property allows us to explore how the model is able to capture higher-order information about the environment and use that information to optimize neural coding and aid the processing of complex visual tasks. Using this model we can make a number of very specific predictions about the mechanistic workings of the brain. Specifically, the model predicts a crucial role of parvalbumin-expressing interneurons in robust development and divisive normalization, while it implicates somatostatin immunoreactive neurons in mediating longer range and feature-selective suppression. The model also makes predictions about the role of these cell classes in efficient neural coding and under what conditions the model fails to organize. In particular, we show that a tight coupling of activity between the principal excitatory population and the parvalbumin population is central to robust and stable responses and organization, which may have implications for a variety of diseases where parvalbumin interneuron function is impaired, such as schizophrenia and autism. Further the model explains the switch from facilitatory to suppressive surround modulation effects as a simple by-product of the facilitating response function of long-range excitatory connections targeting a specialized class of inhibitory interneurons. Finally, the model allows us to make predictions about the statistics that are encoded in the extensive network of long-range intra-areal connectivity in V1, suggesting that even V1 can capture high-level statistical dependencies in the visual environment. The final model represents a comprehensive and well constrained model of the primary visual cortex, which for the first time can relate the physiological properties of individual cell classes to their role in development, learning and function. While the model is specifically tuned for V1, all mechanisms introduced are completely general, and can be used as a general cortical model, useful for studying phenomena across the visual cortex and even the cortex as a whole. This work is also highly relevant for clinical neuroscience, as the cell types studied here have been implicated in neurological disorders as wide ranging as autism, schizophrenia and Parkinson’s disease.

612.8

Analysis of Medicago truncatula transcription factors involved in the arbuscular mycorrhizal symbiosis

Bortfeld, Silvia

January 2013

For the first time the transcriptional reprogramming of distinct root cortex cells during the arbuscular mycorrhizal (AM) symbiosis was investigated by combining Laser Capture Mirodissection and Affymetrix GeneChip® Medicago genome array hybridization. The establishment of cryosections facilitated the isolation of high quality RNA in sufficient amounts from three different cortical cell types. The transcript profiles of arbuscule-containing cells (arb cells), non-arbuscule-containing cells (nac cells) of Rhizophagus irregularis inoculated Medicago truncatula roots and cortex cells of non-inoculated roots (cor) were successfully explored. The data gave new insights in the symbiosis-related cellular reorganization processes and indicated that already nac cells seem to be prepared for the upcoming fungal colonization. The mycorrhizal- and phosphate-dependent transcription of a GRAS TF family member (MtGras8) was detected in arb cells and mycorrhizal roots. MtGRAS shares a high sequence similarity to a GRAS TF suggested to be involved in the fungal colonization processes (MtRAM1). The function of MtGras8 was unraveled upon RNA interference- (RNAi-) mediated gene silencing. An AM symbiosis-dependent expression of a RNAi construct (MtPt4pro::gras8-RNAi) revealed a successful gene silencing of MtGras8 leading to a reduced arbuscule abundance and a higher proportion of deformed arbuscules in root with reduced transcript levels. Accordingly, MtGras8 might control the arbuscule development and life-time. The targeting of MtGras8 by the phosphate-dependent regulated miRNA5204* was discovered previously (Devers et al., 2011). Since miRNA5204* is known to be affected by phosphate, the posttranscriptional regulation might represent a link between phosphate signaling and arbuscule development. In this work, the posttranscriptional regulation was confirmed by mis-expression of miRNA5204* in M. truncatula roots. The miRNA-mediated gene silencing affects the MtGras8 transcript abundance only in the first two weeks of the AM symbiosis and the mis-expression lines seem to mimic the phenotype of MtGras8-RNAi lines. Additionally, MtGRAS8 seems to form heterodimers with NSP2 and RAM1, which are known to be key regulators of the fungal colonization process (Hirsch et al., 2009; Gobbato et al., 2012). These data indicate that MtGras8 and miRNA5204* are linked to the sym pathway and regulate the arbuscule development in phosphate-dependent manner. / Die Leguminose Medicago truncatula (gehört zur Gattung des Schneckenklees) ist in der Lage sowohl eine Symbiose mit stickstofffixierenden Bakterien (Rhizobien), als auch mit Mykorrhiza-Pilzen einzugehen. Der Mykorrhiza-Pilz Rhizophagus irregularis dringt in die Wurzelrindenzellen ein und bildet Strukturen aus, die als Arbuskeln bezeichnet werden. Diese ermöglichen den Transfer von Nährstoffen, wie Phosphat in die Wurzelzellen. Die Pflanze liefert hingegen bis zu 20 % ihrer Photosyntheseprodukte an den Pilz. Da die Lebenszeit der Arbuskeln nur wenige Tage beträgt, können Wurzelrindenzellen mehrere Arbuskeln nacheinander beherbergen. Somit können neben arbuskelhaltigen, auch nicht-arbuskelhaltige Zellen in kolonisierten Wurzeln auftreten. Die nicht-arbuskelhaltigen Zellen beeinträchtigen die Sensitivität von Genregulationsanalysen, wenn die Genregulation während der Mykorrhiza-Symbiose anhand von ganzen kolonisierten Wurzeln untersucht wird. In dieser Arbeit konnte eine Zelltyp-spezifische Analyse der Genregulation von arbuskelhaltigen und nicht-arbuskelhaltigen Zellen durchgeführt, und eine Erhöhung der Sensitivität erreicht werden. Mittels Laser Capture Microdissection wurden Zellen aus Gefrierschnitten von Wurzeln isoliert. Aus den so gewonnen Zellen konnte RNA von ausreichender Qualität und Quantität extrahiert werden, um das Transkriptom der beiden Zelltypen mittels Mikroarrayhybridisierung zu untersuchen. Transkriptionsfaktoren (TFs) spielen wahrscheinlich eine Schlüsselrolle in der Umprogrammierung von Wurzelzellen während der Mykorrhiza-Symbiose. Daher wurde die Genregulation von TF-Genen in den zwei Zelltypen gezielt untersucht. Anhand von quantitativer RT-PCR und Promoter-Reporter-Fusionen wurde die differentielle Expression von mehreren TF-Transkripten in den verschiedenen Zelltypen bestätigt. Die Charakterisierung eines potentiellen GRAS TF (MtGRAS8) konnte eine stark Symbiose- und Phosphat-abhängige Induktion von Transkripten bestätigt werden. Mutanten mit verringerter MtGras8 Transkriptmenge wiesen eine verringerte Arbuskelzahl und deformierte Arbuskeln auf. MtGras8 scheint daher an der Arbuskelentwicklung beteiligt zu sein. Vorherige Experimente zeigten, dass MtGras8 Transkripte, von der Phosphat-regulierten MikroRNA5204* geschnitten werden (Devers et al., 2011). Dies konnte durch Überexpression der MikroRNA5204* in vivo bestätigt werden. Weiterhin konnten Protein-Protein-Interaktionen von MtGras8 mit bekannten GRAS TFs (NSP1, NSP2, RAM1) nachgewiesen und daraus eine Verbindung zu bekannten Symbiose-induzierten Signalkaskaden geschlossen werden. In dieser Arbeit wurde erstmals die Umprogrammierung von nicht-arbuskelhaltigen Zellen untersucht und neue Regulationselemente für die Kontrolle der Arbuskelentwicklung, wie MtGRAS8 und MikroRNA5204*, charakterisiert.

arbuskuläre Mykorrhiza-Symbiose

Transkriptionsfaktoren

Zelltyp-spezifisch

Transkriptomanalyse

arbuscular mycorrhizal symbiosis

transcription factors

cell type-specific

transcriptome analysis

Life sciences

Using cell type-specific methods to understand molecular processes in the brain

Rajput, Ashish

01 June 2018

No description available.

610

cell type-specific methods

Epigenetics

Learning and memory

DNA methylation

Tagger mouse

Single cell sequencing

Drop-seq

Aging

in-vivo method

motor neurons

Neurogenesis

Molecular Medicine