Your search keyword '"Benjamin Titze"' showing total 12 results

1. Fast Homogeneous En Bloc Staining of Large Tissue Samples for Volume Electron Microscopy

Author

Christel Genoud, Benjamin Titze, Alexandra Graff-Meyer, and Rainer W. Friedrich

Subjects

EM, protocol, BROPA, connectomics, SBEM, block-face, Neurosciences. Biological psychiatry. Neuropsychiatry, RC321-571, Human anatomy, QM1-695

Abstract

Fixation and staining of large tissue samples are critical for the acquisition of volumetric electron microscopic image datasets and the subsequent reconstruction of neuronal circuits. Efficient protocols exist for the staining of small samples, but uniform contrast is often difficult to achieve when the sample diameter exceeds a few hundred micrometers. Recently, a protocol (BROPA, brain-wide reduced-osmium staining with pyrogallol-mediated amplification) was developed that achieves homogeneous staining of the entire mouse brain but requires very long sample preparation times. By exploring modifications of this protocol we developed a substantially faster procedure, fBROPA, that allows for reliable high-quality staining of tissue blocks on the millimeter scale. Modifications of the original BROPA protocol include drastically reduced incubation times and a lead aspartate incubation to increase sample conductivity. Using this procedure, whole brains from adult zebrafish were stained within 4 days. Homogenous high-contrast staining was achieved throughout the brain. High-quality image stacks with voxel sizes of 10 × 10 × 25 nm3 were obtained by serial block-face imaging using an electron dose of ~15 e−/nm2. No obvious reduction in staining quality was observed in comparison to smaller samples stained by other state-of-the-art procedures. Furthermore, high-quality images with minimal charging artifacts were obtained from non-neural tissues with low membrane density. fBROPA is therefore likely to be a versatile and efficient sample preparation protocol for a wide range of applications in volume electron microscopy.

Published

2018

2. SBEMimage: Versatile Acquisition Control Software for Serial Block-Face Electron Microscopy

Author

Benjamin Titze, Christel Genoud, and Rainer W. Friedrich

Subjects

SBEM, imaging software, connectomics, serial block-face, SEM, volume EM, Neurosciences. Biological psychiatry. Neuropsychiatry, RC321-571

Abstract

We present SBEMimage, an open-source Python-based application to operate serial block-face electron microscopy (SBEM) systems. SBEMimage is designed for complex, challenging acquisition tasks, such as large-scale volume imaging of neuronal tissue or other biological ultrastructure. Advanced monitoring, process control, and error handling capabilities improve reliability, speed, and quality of acquisitions. Debris detection, autofocus, real-time image inspection, and various other quality control features minimize the risk of data loss during long-term acquisitions. Adaptive tile selection allows for efficient imaging of large tissue volumes of arbitrary shape. The software’s graphical user interface is optimized for remote operation. In its user-friendly viewport, tile grids covering the region of interest to be acquired are overlaid on previously acquired overview images of the sample surface. Images from other sources, e.g., light microscopes, can be imported and superimposed. SBEMimage complements existing DigitalMicrograph (Gatan Microscopy Suite) installations on 3View systems but permits higher acquisition rates by interacting directly with the microscope’s control software. Its modular architecture and the use of Python/PyQt make SBEMimage highly customizable and extensible, which allows for fast prototyping and will permit adaptation to a wide range of SBEM systems and applications.

Published

2018

3. Author Correction: Volume electron microscopy

Author

Christopher J. Peddie, Christel Genoud, Anna Kreshuk, Kimberly Meechan, Kristina D. Micheva, Kedar Narayan, Constantin Pape, Robert G. Parton, Nicole L. Schieber, Yannick Schwab, Benjamin Titze, Paul Verkade, Aubrey Weigel, and Lucy M. Collinson

Subjects

General Medicine, General Chemistry

Published

2022

4. Volume electron microscopy

Author

Christopher J. Peddie, Christel Genoud, Anna Kreshuk, Kimberly Meechan, Kristina D. Micheva, Kedar Narayan, Constantin Pape, Robert G. Parton, Nicole L. Schieber, Yannick Schwab, Benjamin Titze, Paul Verkade, Aubrey Weigel, and Lucy M. Collinson

Subjects

General Medicine, General Biochemistry, Genetics and Molecular Biology

Published

2022

5. Whole-body integration of gene expression and single-cell morphology

Author

Emily L. Savage, Oleg Simakov, Anna Kreshuk, Pedro Machado, Christian Tischer, Valentyna Zinchenko, Kimberly Meechan, Yannick Schwab, Rainer W. Friedrich, Paola Bertucci, Benjamin Titze, Detlev Arendt, Rachel M. Templin, Christel Genoud, Hernando Martínez Vergara, Constantin Pape, and Adrian A. Wanner

Subjects

0303 health sciences, Cell type, Effector, Cell, Computational biology, Biology, Cell morphology, 03 medical and health sciences, 0302 clinical medicine, medicine.anatomical_structure, Cytoarchitecture, Gene expression, medicine, 14. Life underwater, Gene, Transcription factor, 030217 neurology & neurosurgery, 030304 developmental biology

Abstract

SummaryAnimal bodies are composed of hundreds of cell types that differ in location, morphology, cytoarchitecture, and physiology. This is reflected by cell type-specific transcription factors and downstream effector genes implementing functional specialisation. Here, we establish and explore the link between cell type-specific gene expression and subcellular morphology for the entire body of the marine annelidPlatynereis dumerilii. For this, we registered a whole-body cellular expression atlas to a high-resolution electron microscopy dataset, automatically segmented all cell somata and nuclei, and clustered the cells according to gene expression or morphological parameters. We show that collective gene expression most efficiently identifies spatially coherent groups of cells that match anatomical boundaries, which indicates that combinations of regionally expressed transcription factors specify tissue identity. We provide an integrated browser as a Fiji plugin to readily explore, analyse and visualise multimodal datasets with remote on-demand access to all available datasets.

Published

2020

6. Whole Body Integration of Gene Expression and Morphology Using Correlative Volume EM

Author

Rainer W. Friedrich, Oleg Simakov, Emily L. Savage, Pedro Machado, Hernando Martínez Vergara, Anna Kreshuk, Valentyna Zinchenko, Constantin Pape, Christel Genoud, Christian Tischer, Adrian A. Wanner, Kimberly Meechan, Yannick Schwab, Rachel M. Templin, Benjamin Titze, Paola Betucci, and Detlev Arendt

Subjects

Correlative, Morphology (linguistics), Volume (thermodynamics), Gene expression, Biology, Whole body, Instrumentation, Cell biology

Published

2020

7. Volume scanning electron microscopy for imaging biological ultrastructure

Author

Christel Genoud and Benjamin Titze

Subjects

0301 basic medicine, Histocytological Preparation Techniques, Scanning electron microscope, Cellular imaging, Cell Biology, General Medicine, Biology, Focused ion beam, law.invention, 03 medical and health sciences, 030104 developmental biology, law, Microtome, Ultrastructure, Biophysics, Electron microscope, Biomedical engineering, Volume (compression)

Abstract

Electron microscopy (EM) has been a key imaging method to investigate biological ultrastructure for over six decades. In recent years, novel volume EM techniques have significantly advanced nanometre-scale imaging of cells and tissues in three dimensions. Previously, this had depended on the slow and error-prone manual tasks of cutting and handling large numbers of sections, and imaging them one-by-one with transmission EM. Now, automated volume imaging methods mostly based on scanning EM (SEM) allow faster and more reliable acquisition of serial images through tissue volumes and achieve higher z-resolution. Various software tools have been developed to manipulate the acquired image stacks and facilitate quantitative analysis. Here, we introduce three volume SEM methods: serial block-face electron microscopy (SBEM), focused ion beam SEM (FIB-SEM) and automated tape-collecting ultramicrotome SEM (ATUM-SEM). We discuss and compare their capabilities, provide an overview of the full volume SEM workflow for obtaining 3D datasets and showcase different applications for biological research.

Published

2016

8. Fast Homogeneous En Bloc Staining of Large Tissue Samples for Volume Electron Microscopy

Author

Alexandra Graff-Meyer, Benjamin Titze, Rainer W. Friedrich, and Christel Genoud

Subjects

0301 basic medicine, Materials science, Sample (material), block-face, Neuroscience (miscellaneous), computer.software_genre, law.invention, lcsh:RC321-571, lcsh:QM1-695, 03 medical and health sciences, Cellular and Molecular Neuroscience, 0302 clinical medicine, Voxel, law, Methods, Sample preparation, protocol, connectomics, lcsh:Neurosciences. Biological psychiatry. Neuropsychiatry, Fixation (histology), sample preparation, lcsh:Human anatomy, zebrafish, Staining, BROPA, 030104 developmental biology, Homogeneous, EM, SBEM, Electron microscope, Anatomy, computer, 030217 neurology & neurosurgery, Volume (compression), Biomedical engineering, Neuroscience

Abstract

Fixation and staining of large tissue samples are critical for the acquisition of volumetric electron microscopic image datasets and the subsequent reconstruction of neuronal circuits. Efficient protocols exist for the staining of small samples, but uniform contrast is often difficult to achieve when the sample diameter exceeds a few hundred micrometers. Recently, a protocol (BROPA, brain-wide reduced-osmium staining with pyrogallol-mediated amplification) was developed that achieves homogeneous staining of the entire mouse brain but requires very long sample preparation times. By exploring modifications of this protocol we developed a substantially faster procedure, fBROPA, that allows for reliable high-quality staining of tissue blocks on the millimeter scale. Modifications of the original BROPA protocol include drastically reduced incubation times and a lead aspartate incubation to increase sample conductivity. Using this procedure, whole brains from adult zebrafish were stained within 4 days. Homogenous high-contrast staining was achieved throughout the brain. High-quality image stacks with voxel sizes of 10 × 10 × 25 nm3 were obtained by serial block-face imaging using an electron dose of ~15 e-/nm2. No obvious reduction in staining quality was observed in comparison to smaller samples stained by other state-of-the-art procedures. Furthermore, high-quality images with minimal charging artifacts were obtained from non-neural tissues with low membrane density. fBROPA is therefore likely to be a versatile and efficient sample preparation protocol for a wide range of applications in volume electron microscopy.

Published

2018

9. A versatile en bloc staining procedure for large volume sample imaging

Author

Alexandra, Graff Meyer, primary, Benjamin, Titze, additional, and Christel, Genoud, additional

Published

2019

10. Automated in-chamber specimen coating for serial block-face electron microscopy

Author

Benjamin Titze and Winfried Denk

Subjects

Histology, Materials science, Microscope, business.industry, Scanning electron microscope, engineering.material, Focused ion beam, Pathology and Forensic Medicine, law.invention, Optics, Coating, law, Microscopy, Microtome, engineering, Diamond knife, Electron microscope, business

Abstract

When imaging insulating specimens in a scanning electron microscope, negative charge accumulates locally ('sample charging'). The resulting electric fields distort signal amplitude, focus and image geometry, which can be avoided by coating the specimen with a conductive film prior to introducing it into the microscope chamber. This, however, is incompatible with serial block-face electron microscopy (SBEM), where imaging and surface removal cycles (by diamond knife or focused ion beam) alternate, with the sample remaining in place. Here we show that coating the sample after each cutting cycle with a 1-2 nm metallic film, using an electron beam evaporator that is integrated into the microscope chamber, eliminates charging effects for both backscattered (BSE) and secondary electron (SE) imaging. The reduction in signal-to-noise ratio (SNR) caused by the film is smaller than that caused by the widely used low-vacuum method. Sample surfaces as large as 12 mm across were coated and imaged without charging effects at beam currents as high as 25 nA. The coatings also enabled the use of beam deceleration for non-conducting samples, leading to substantial SNR gains for BSE contrast. We modified and automated the evaporator to enable the acquisition of SBEM stacks, and demonstrated the acquisition of stacks of over 1000 successive cut/coat/image cycles and of stacks using beam deceleration or SE contrast.

Published

2013

11. Volume scanning electron microscopy for imaging biological ultrastructure

Author

Benjamin, Titze and Christel, Genoud

Subjects

Histocytological Preparation Techniques, Image Processing, Computer-Assisted, Microscopy, Electron, Scanning, Animals, Brain, Humans, Microtomy

Abstract

Electron microscopy (EM) has been a key imaging method to investigate biological ultrastructure for over six decades. In recent years, novel volume EM techniques have significantly advanced nanometre-scale imaging of cells and tissues in three dimensions. Previously, this had depended on the slow and error-prone manual tasks of cutting and handling large numbers of sections, and imaging them one-by-one with transmission EM. Now, automated volume imaging methods mostly based on scanning EM (SEM) allow faster and more reliable acquisition of serial images through tissue volumes and achieve higher z-resolution. Various software tools have been developed to manipulate the acquired image stacks and facilitate quantitative analysis. Here, we introduce three volume SEM methods: serial block-face electron microscopy (SBEM), focused ion beam SEM (FIB-SEM) and automated tape-collecting ultramicrotome SEM (ATUM-SEM). We discuss and compare their capabilities, provide an overview of the full volume SEM workflow for obtaining 3D datasets and showcase different applications for biological research.

Published

2016

12. Whole-body integration of gene expression and single-cell morphology

Author

Lothar Schermelleh, Benjamin Titze, Rachel M. Templin, Anna Kreshuk, Christian Tischer, Kimberly Meechan, Yannick Schwab, Kevin Nzumbi Mutemi, Emily L. Savage, Hernando Martínez Vergara, Detlev Arendt, Constantin Pape, Adrian A. Wanner, Rainer W. Friedrich, Oleg Simakov, Valentyna Zinchenko, Wiebke Dürichen, Paola Bertucci, Pedro Machado, and Christel Genoud

Subjects

Resource, Cell type, Cell, Animals, Cell Nucleus/metabolism, Cell Shape, Ganglia, Invertebrate/metabolism, Gene Expression Profiling, Gene Expression Regulation, Multigene Family, Multimodal Imaging, Mushroom Bodies/metabolism, Polychaeta/cytology, Polychaeta/genetics, Polychaeta/ultrastructure, Single-Cell Analysis, Platynereis dumerilii, automatic segmentation, cell types, gene expression atlas, image registration, machine learning, multimodal data integration, mushroom bodies, telencephalon, volume electron microscopy, Computational biology, Biology, Cell morphology, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, 0302 clinical medicine, Gene expression, medicine, Whole Body Imaging, Mushroom Bodies, 030304 developmental biology, Cell Nucleus, Regulation of gene expression, 0303 health sciences, Cerebrum, Polychaeta, Ganglia, Invertebrate, Chromatin, medicine.anatomical_structure, Positron-Emission Tomography, Mushroom bodies, 030217 neurology & neurosurgery

Abstract

Summary Animal bodies are composed of cell types with unique expression programs that implement their distinct locations, shapes, structures, and functions. Based on these properties, cell types assemble into specific tissues and organs. To systematically explore the link between cell-type-specific gene expression and morphology, we registered an expression atlas to a whole-body electron microscopy volume of the nereid Platynereis dumerilii. Automated segmentation of cells and nuclei identifies major cell classes and establishes a link between gene activation, chromatin topography, and nuclear size. Clustering of segmented cells according to gene expression reveals spatially coherent tissues. In the brain, genetically defined groups of neurons match ganglionic nuclei with coherent projections. Besides interneurons, we uncover sensory-neurosecretory cells in the nereid mushroom bodies, which thus qualify as sensory organs. They furthermore resemble the vertebrate telencephalon by molecular anatomy. We provide an integrated browser as a Fiji plugin for remote exploration of all available multimodal datasets., Graphical abstract, Highlights • A cellular atlas integrates gene expression and ultrastructure for an entire annelid • Morphometry of all segmented cells, nuclei, and chromatin categorizes cell classes • Molecular anatomy and projectome of head ganglionic nuclei and mushroom bodies • An open-source browser for multimodal big image data exploration and analysis, A framework for integrating cellular-resolution gene expression and cell morphological information at full-organism scale is provided for the marine annelid Platynereis dumerilii