Agradecemos a Paavo Bergmann, Michael Laumann, e Sebastian Schmelzle por sua ajuda no ESRF. Este trabalho foi financiado pelo projecto European Synchrotron Radiation Facility SC-2127 através da alocação de tempo de feixe.

Animais utilizados neste estudo Exemplares do ácaro oribatídeos partenogenéticos Archegozetes longisetosus (Acari, Oribatida) foram retirados de nossa cultura em laboratório. A cultura cresce em um gesso de Paris / mix de carvão vegetal (9:1) em frascos de plástico, no escuro constante em 20-23 ° C, com aproximadamente 90% da umidade do ar. Preparação de amostras <ol><li> Espécimes foram retirados a partir da cultura, limpo com um pincel fino e colocado em uma mistura de etanol 06:03:01 80%, de formaldeído 35% e 100% de ácido acético por 24 horas. </li><li> Posteriormente, as amostras foram desidratadas em uma série de etanol graduada de 70%, 75%, 80%, 85%, 90%, 95% e 100% com 3 alterações em cada concentração, e 10 min entre as etapas. </li><li> Finalmente, as amostras foram colocadas no ponto de etanol 100% durante a noite fresca e crítica secas em CO 2 (CPD 020, Balzers). Amostras secas foram anexados à ponta de pinos plásticos (1,2 cm de comprimento, 3,0 mm de diâmetro). </li></ol> Síncrotron de raios-X a tomografia X-ray tomografia foi realizada na linha de luz ID19 (ESRF, Grenoble, França, experiência SC-2127). <ol><li> As amostras foram montadas no porta-amostras e ajustada para uma posição central na viga. </li><li> As amostras foram medidas com uma energia de 20,5 keV. As radiografias foram gravados com um CCD refrigerado (ESRF Frelon câmera) com uma gama dinâmica de 14 bits, 2048 × 2048 pixels e um tamanho de pixel efetiva de 0,7 mM. 1500 foram registrados projeções sobre a rotação da amostra 180 ° com um tempo de exposição de 0,35 s para cada projeção. A distância detector-de-amostra foi de 20 mm. </li></ol> Usando uma certa distância entre a amostra eo detector permite uma imagem diferencial de materiais com baixos coeficientes de atenuação de raios-X (Cloetens, et al. 1996), o que produziria contraste insuficiente em imagem de absorção (onde a amostra é localizado diretamente em frente ao detector ). Assuntos mais biológicos são objetos fase, composta de materiais com baixa absorção e / ou apenas pequenas diferenças no número atômico (Betz, et al. 2007). No entanto, a fase de maior tomografia exige uma coerência alta espacial de um feixe de raios-X homogênea. Portanto, a radiação síncrotron é mais adequado do que desktop-scanners para este tipo de medidas. Análise de dados <ol><li> As radiografias resultantes foram transformados em 2D para 3D de dados voxel (8 bits de cinza valores) com um algoritmo de retro-projeção filtrada (Cloetens, et al., 1997) </li><li> Os dados voxel foram analisadas com o software Max vgstudio 1.2.1. (Graphics Volume, Heidelberg, Alemanha). </li><li> Grey-valores do fundo foram retirados do histograma para visualização 3D. </li><li> Pré-definidos câmera caminhos foram usados ​​para gerar animações de rotação e planos de recorte animado. </li><li> Um user-defined caminho de câmera foi gerada a seguir o sistema digestivo de A. longisetosus. </li></ol>

<ol>
	<li>Betz, O., Wegst, U., Weide, D., Heethoff, M., Helfen, L., Lee, W. -. K., Cloetens, P. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Imaging+applications+of+synchrotron+X-ray+phase-contrast+microtomography+in+biological+morphology+and+biomaterial+science.+I.+General+aspects+of+the+technique+and+its+advantages+in+the+analysis+of+millimetre-sized+arthropod+structure.">Imaging applications of synchrotron X-ray phase-contrast microtomography in biological morphology and biomaterial science. I. General aspects of the technique and its advantages in the analysis of millimetre-sized arthropod structure.</a> J. Microscopy. 22, 51-71 (2007).</li><li>Cloetens, P., Barrett, R., Baruchel, J., Guigay, J. P., Schlenker, M. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Phase+objects+in+synchrotron+radiation+hard+X-ray+imaging.">Phase objects in synchrotron radiation hard X-ray imaging.</a> J. Phys. D: Appl. Phys. 29, 133-146 (1996).</li><li>Cloetens, P., Pateyron-Salome, M., Buffiere, J. Y., Peix, G., Baruchel, J., Peyrin, V., Schlenker, M. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Observation+in+microstructure+and+damage+in+materials+by+phase+sensitive+radiography+and+tomography.">Observation in microstructure and damage in materials by phase sensitive radiography and tomography.</a> J. Apll. Phys. 81, 5878-5886 (1997).</li><li>Clotens, P., Ludwig, W., Baruchel, J., van Dyck, D., van Landyut, J., Guigay, J. P., Schlenker, M. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Holotomography:+quantitative+phase+tomography+with+micrometer+resolution+using+hard+synchrotron+radiation+X-rays.">Holotomography: quantitative phase tomography with micrometer resolution using hard synchrotron radiation X-rays.</a> Appl. Phys. Lett. 75, 2912-2914 (1999).</li><li>Heethoff, M., Cloetens, P. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=A+Comparison+of+aynchrotron+X-ray+phase+contrast+tomography+and+holotomography+for+non-invasive+investigations+of+the+internal+anatomy+of+mites.">A Comparison of aynchrotron X-ray phase contrast tomography and holotomography for non-invasive investigations of the internal anatomy of mites.</a> Soil Organisms. , (2008).</li></ol>

The authors have nothing to disclose.

Nesta apresentação, nós nos concentramos na visualização 3D da anatomia interna de um chelicerate micro-artrópodes. O síncrotron de raios-X medidas permitem que um pixel de resolução de até 0.3μm, dependendo do tamanho da amostra. Aqui, mostramos dados com 0.7μm pixels de resolução. Geralmente, síncrotron tomografia de raios-X pode ser útil para analisar pequenas material biológico (ou tecidos), com atenuação de raios-X de baixa. O pixel de resolução quase alcança o de microscopia de luz convencional. A técnica pode s...

non-invasive 3d-visualization with sub-micron resolution using synchrotron-x-ray-tomography

Pouco se sabe sobre a organização interna de muitos micro-artrópodes com tamanhos de corpo abaixo de 1 mm. As razões para isso são o pequeno tamanho ea cutícula dura que o torna difícil de usar protocolos de histologia clássica. Além disso, o corte histológico destrói a amostra e portanto, não pode ser usado para o material original. Assim, um método não-destrutivo é desejável que permite visão interna de pequenas amostras sem a necessidade de corte. Usamos síncrotron tomografia de raios-X no Laboratório Europeu de Radiação Síncrotron (ESRF) em Grenoble (França) para não-invasiva produzir conjuntos de dados 3D tomográficos com um pixel de resolução de 0.7μm. Usando software de renderização de volume, o que nos permite reconstruir a organização interna em seu estado natural, sem os artefatos produzidos por corte histológico. Estas datas podem ser usados ​​para a morfologia quantitativa, marcos, ou para a visualização de filmes de animação para compreender a estrutura de partes do corpo escondido e seguir sistemas de órgãos ou tecidos completa através das amostras.

Watch this Scientific Journal Video about Non-invasive 3D-Visualization with Sub-micron Resolution Using Synchrotron-X-ray-tomography at JoVE.com

Non-invasive 3D-Visualization with Sub-micron Resolution Using Synchrotron-X-ray-tomography

Usamos síncrotron tomografia de raios-X no Laboratório Europeu de Radiação Síncrotron (ESRF) para não-invasiva produzir conjuntos de dados 3D tomográficos com um pixel de resolução de 0.7μm. Usando software de renderização de volume, o que permite a reconstrução de estruturas internas em seu estado natural, sem os artefatos produzidos por corte histológico.

Não-invasivo 3D Visualization com Sub-micron Resolução Usando Síncrotron-X-ray-tomografia

Little is known about the internal organization of many micro-arthropods with body sizes below 1 mm. The reasons for that are the small size and the hard ...

non-invasive-3d-visualization-with-sub-micron-resolution-using

Research

JoVE Journal

Biology

13.0K visualizações.  University of Tubingen. Usamos síncrotron tomografia de raios-X no Laboratório Europeu de Radiação Síncrotron (ESRF) para não-invasiva produzir conjuntos de dados 3D tomográficos com um pixel de resolução de 0.7μm. Usando software de renderização de volume, o que permite a reconstrução de estruturas internas em seu estado natural, sem os artefatos produzidos por corte histológico.

Vídeo: Non-invasive 3D-Visualization with Sub-micron Resolution Using Synchrotron-X-ray-tomography

Labeling hESCs and hMSCs with Iron Oxide Nanoparticles for Non-Invasive in vivo Tracking with MR Imaging

In recent years, stem cell research has led to a better understanding of developmental biology, various diseases and its potential impact on regenerative medicine. A non-invasive method to monitor the transplanted stem cells repeatedly in vivo would greatly enhance our ability to understand the mechanisms that control stem cell death and identify trophic factors and signaling pathways that improve stem cell engraftment. MR imaging has been proven to be an effective tool for the in vivo depiction of stem cells with near microscopic anatomical resolution. In order to detect stem cells with MR, the cells have to be labeled with cell specific MR contrast agents. For this purpose, iron oxide nanoparticles, such as superparamagnetic iron oxide particles (SPIO), are applied, because of their high sensitivity for cell detection and their excellent biocompatibility. SPIO particles are composed of an iron oxide core and a dextran, carboxydextran or starch coat, and function by creating local field inhomogeneities, that cause a decreased signal on T2-weighted MR images. This presentation will demonstrate techniques for labeling of stem cells with clinically applicable MR contrast agents for subsequent non-invasive in vivo tracking of the labeled cells with MR imaging.

For the evaluation of new stem cell therapies it is important to non-invasively track the injected cells in vivo. This video will show you how to label human mesenchymal and embryonic stem cells with iron oxide based contrast agents in vivo for subsequent MR imaging in vivo.

Rotulagem e hESCs hMSCs com óxido de ferro nanopartículas para Não-invasiva em Rastreamento vivo com ressonância magnética

In recent years, stem cell research has led to a better understanding of developmental biology, various diseases and its potential impact on regenerative ...

Biologia

Labeling Stem Cells with Fluorescent Dyes for non-invasive Detection with Optical Imaging

Optical imaging (OI) is an easy, fast and inexpensive tool for in vivo monitoring of new stem cell based therapies. The technique is based on ex vivo labeling of stem cells with a fluorescent dye, subsequent intravenous injection of the labeled cells and visualization of their accumulation in specific target organs or pathologies. The presented technique demonstrates how we label human mesenchymal stem cells (hMSC) by simple incubation with the lipophilic fluorescent dye DiD (C67H103CIN2O3S) and how we label human embryonic stem cells (hESC) with the FDA approved fluorescent dye Indocyanine Green (ICG). The uptake mechanism is via adherence and diffusion of the lypophilic dye across the phospholipid cell membrane bilayer. The labeling efficiency is usually improved if the cells are incubated with the dye in serum-free media as opposed to incubation in serum-containing media. Furthermore, the addition of the transfection agent Protamine Sulfate significantly improves contrast agent uptake.

This video shows techniques for labeling of human embryonic stem cells and mesenchymal stem cells with fluorescent dyes. This technique can be used for an in vivo tracking of transplanted stem cells with optical imaging and for histopathological correlations with fluorescence microscopy.

Rotulagem células-tronco com corantes fluorescentes para detecção não invasiva com imagens ópticas

Optical imaging (OI) is an easy, fast and inexpensive tool for in vivo monitoring of new stem cell based therapies. The technique is based on ex vivo ...

A Reversible, Non-invasive Method for Airway Resistance Measurements and Bronchoalveolar Lavage Fluid Sampling in Mice

Airway hyperreactivity (AHR) measurements and bronchoalveolar lavage (BAL) fluid sampling are essential to experimental asthma models, but repeated procedures to obtain such measurements in the same animal are generally not feasible.  Here, we demonstrate protocols for obtaining from mice repeated measurements of AHR and bronchoalveolar lavage fluid samples.  Mice were challenged intranasally seven times over 14 days with a potent allergen or sham treated.  Prior to the initial challenge, and within 24 hours following each intranasal challenge, the same animals were anesthetized, orally intubated and mechanically ventilated.  AHR, assessed by comparing dose response curves of respiratory system resistance (RRS) induced by increasing intravenous doses of acetylcholine (Ach) chloride between sham and allergen-challenged animals, were determined.  Afterwards, and via the same intubation, the left lung was lavaged so that differential enumeration of airway cells could be performed.  These studies reveal that repeated measurements of AHR and BAL fluid collection are possible from the same animals and that maximal airway hyperresponsiveness and airway eosinophilia are achieved within 7-10 days of initiating allergen challenge.  This novel technique significantly reduces the number of mice required for longitudinal experimentation and is applicable to diverse rodent species, disease models and airway physiology instruments.  

Repeated measurements of rodent respiratory physiology and sampling of airway inflammatory cells are desirable, but generally not feasible. Here we describe a repeatable method for orally intubating mice that permits repeated measurements of airway hyperreactivity and sampling of airway inflammatory cells.

A reversível, método não-invasivo para medições de Resistência das Vias Aéreas e Amostragem Líquido da Lavagem Broncoalveolar em Ratos

Airway hyperreactivity (AHR) measurements and bronchoalveolar lavage (BAL) fluid sampling are essential to experimental asthma models, but repeated ...

iCLIP - Transcriptome-wide Mapping of Protein-RNA Interactions with Individual Nucleotide Resolution

The unique composition and spatial arrangement of RNA-binding proteins (RBPs) on a transcript guide the diverse aspects of post-transcriptional regulation1. Therefore, an essential step towards understanding transcript regulation at the molecular level is to gain positional information on the binding sites of RBPs2.
Protein-RNA interactions can be studied using biochemical methods, but these approaches do not address RNA binding in its native cellular context. Initial attempts to study protein-RNA complexes in their cellular environment employed affinity purification or immunoprecipitation combined with differential display or microarray analysis (RIP-CHIP)3-5. These approaches were prone to identifying indirect or non-physiological interactions6. In order to increase the specificity and positional resolution, a strategy referred to as CLIP (UV cross-linking and immunoprecipitation) was introduced7,8. CLIP combines UV cross-linking of proteins and RNA molecules with rigorous purification schemes including denaturing polyacrylamide gel electrophoresis. In combination with high-throughput sequencing technologies, CLIP has proven as a powerful tool to study protein-RNA interactions on a genome-wide scale (referred to as HITS-CLIP or CLIP-seq)9,10. Recently, PAR-CLIP was introduced that uses photoreactive ribonucleoside analogs for cross-linking11,12.
Despite the high specificity of the obtained data, CLIP experiments often generate cDNA libraries of limited sequence complexity. This is partly due to the restricted amount of co-purified RNA and the two inefficient RNA ligation reactions required for library preparation. In addition, primer extension assays indicated that many cDNAs truncate prematurely at the crosslinked nucleotide13. Such truncated cDNAs are lost during the standard CLIP library preparation protocol. We recently developed iCLIP (individual-nucleotide resolution CLIP), which captures the truncated cDNAs by replacing one of the inefficient intermolecular RNA ligation steps with a more efficient intramolecular cDNA circularization (Figure 1)14. Importantly, sequencing the truncated cDNAs provides insights into the position of the cross-link site at nucleotide resolution. We successfully applied iCLIP to study hnRNP C particle organization on a genome-wide scale and assess its role in splicing regulation14.

The spatial arrangement of RNA-binding proteins on a transcript is a key determinant of post-transcriptional regulation. Therefore, we developed individual-nucleotide resolution UV crosslinking and immunoprecipitation (iCLIP) that allows precise genome-wide mapping of the binding sites of an RNA-binding protein.

iCLIP - Transcriptoma-wide Mapeamento das Interações Proteína-RNA com a Resolução Nucleotide Individual

The unique composition and spatial arrangement of RNA-binding proteins (RBPs) on a transcript guide the diverse aspects of post-transcriptional ...

Rapid and Efficient Zebrafish Genotyping Using PCR with High-resolution Melt Analysis

Zebrafish is a powerful vertebrate model system for studying development, modeling disease, and performing drug screening. Recently a variety of genetic tools have been introduced, including multiple strategies for inducing mutations and generating transgenic lines. However, large-scale screening is limited by traditional genotyping methods, which are time-consuming and labor-intensive. Here we describe a technique to analyze zebrafish genotypes by PCR combined with high-resolution melting analysis (HRMA).&#160;This approach is rapid, sensitive, and inexpensive, with lower risk of contamination artifacts.&#160;Genotyping by PCR with HRMA can be used for embryos or adult fish, including in high-throughput screening protocols.

PCR combined with high-resolution melt analysis (HRMA) is demonstrated as a rapid and efficient method to genotype zebrafish.

Rápida e eficiente Zebrafish Genotipagem Usando PCR com alta resolução Análise Melt

Zebrafish is a powerful vertebrate model system for studying development, modeling disease, and performing drug screening. Recently a variety of genetic ...

Who is Who? Non-invasive Methods to Individually Sex and Mark Altricial Chicks

Many experiments require early determination of offspring's sex as well as early marking of newborns for individual recognition. According to animal welfare guidelines, non-invasive techniques should be preferred whenever applicable. In our group, we work on different species of song birds in the lab and in the field, and we successfully apply non-invasive methods to sex and individually mark chicks. This paper presents a comprehensive non-invasive tool-box. Sexing birds prior to the expression of secondary sexual traits requires the collection of DNA-bearing material for PCR. We established a quick and easy method to sex birds of any age (post hatching) by extracting DNA from buccal swabs. Results can be obtained within 3 hours. For individual marking chick's down feathers are trimmed in specific patterns allowing fast identification within the hatching order. This set of methods is easily applicable in a standard equipped lab and especially suitable for working in the field as no special equipment is required for sampling and storage. Handling of chicks is minimized and marking and sexing techniques are non-invasive thereby supporting the RRR-principle of animal welfare guidelines.

This protocol provides a convenient set of methods, which enables extremely fast, easy, non-invasive, reliable and low-cost, molecular sex determination of birds and their non-invasive, quick, safe and easily recognizable marking shortly after hatching. Only limited handling of chicks is required. This convenient toolbox of methods complies entirely with the RRR-guidelines.

Quem é Quem? Métodos não-invasivos para Individualmente Sexo e Mark altriciais Chicks

Many experiments require early determination of offspring's sex as well as early marking of newborns for individual recognition. According to animal ...

Fecal Glucocorticoid Analysis: Non-invasive Adrenal Monitoring in Equids

Adrenal activity can be assessed in the equine species by analysis of feces for corticosterone metabolites. During a potentially aversive situation, corticotrophin releasing hormone (CRH) is released from the hypothalamus in the brain. This stimulates the release of adrenocorticotrophic hormone (ACTH) from the pituitary gland, which in turn stimulates release of glucocorticoids from the adrenal gland. In horses the glucocorticoid corticosterone is responsible for several adaptations needed to support equine flight behaviour and subsequent removal from the aversive situation. Corticosterone metabolites can be detected in the feces of horses and assessment offers a non-invasive option to evaluate long term patterns of adrenal activity. Fecal assessment offers advantages over other techniques that monitor adrenal activity including blood plasma and saliva analysis. The non-invasive nature of the method avoids sampling stress which can confound results. It also allows the opportunity for repeated sampling over time and is ideal for studies in free ranging horses. This protocol describes the enzyme linked immunoassay (EIA) used to assess feces for corticosterone, in addition to the associated biochemical validation.

Adrenal activity can be assessed in the equine species by analysis of feces for corticosterone metabolites. The method offers a non-invasive option to assess long term patterns in both domestic and free ranging horses. This protocol describes the enzyme linked immunoassay involved and the associated biochemical validation.

Fecal Análise de glicocorticóides: Non-invasive Monitoring Adrenal em eqüídeos

Adrenal activity can be assessed in the equine species by analysis of feces for corticosterone metabolites. During a potentially aversive situation, ...

Open-source Single-particle Analysis for Super-resolution Microscopy with VirusMapper

Super-resolution fluorescence microscopy is currently revolutionizing cell biology research. Its capacity to break the resolution limit of around 300 nm allows for the routine imaging of nanoscale biological complexes and processes. This increase in resolution also means that methods popular in electron microscopy, such as single-particle analysis, can readily be applied to super-resolution fluorescence microscopy. By combining this analytical approach with super-resolution optical imaging, it becomes possible to take advantage of the molecule-specific labeling capacity of fluorescence microscopy to generate structural maps of molecular elements within a metastable structure. To this end, we have developed a novel algorithm &#8212; VirusMapper &#8212; packaged as an easy-to-use, high-performance, and high-throughput ImageJ plugin. This article presents an in-depth guide to this software, showcasing its ability to uncover novel structural features in biological molecular complexes. Here, we present how to assemble compatible data and provide a step-by-step protocol on how to use this algorithm to apply single-particle analysis to super-resolution images.

This manuscript uses the Fiji-based open-source software package VirusMapper to apply single-particle analysis to super-resolution microscopy images in order to generate precise models of nanoscale structure.

Análise de partícula única open-source para Microscopia Super-resolução com VirusMapper

Super-resolution fluorescence microscopy is currently revolutionizing cell biology research. Its capacity to break the resolution limit of around 300 nm ...

Analysis of Beta-cell Function Using Single-cell Resolution Calcium Imaging in Zebrafish Islets

Pancreatic beta-cells respond to increasing blood glucose concentrations by secreting the hormone insulin. The dysfunction of beta-cells leads to hyperglycemia and severe, life-threatening consequences. Understanding how the beta-cells operate under physiological conditions and what genetic and environmental factors might cause their dysfunction could lead to better treatment options for diabetic patients. The ability to measure calcium levels in beta-cells serves as an important indicator of beta-cell function, as the influx of calcium ions triggers insulin release. Here we describe a protocol for monitoring the glucose-stimulated calcium influx in zebrafish beta-cells by using GCaMP6s, a genetically encoded sensor of calcium. The method allows monitoring the intracellular calcium dynamics with single-cell resolution in ex vivo mounted islets. The glucose-responsiveness of beta-cells within the same islet can be captured simultaneously under different glucose concentrations, which suggests the presence of functional heterogeneity among zebrafish beta-cells. Furthermore, the technique provides high temporal and spatial resolution, which reveals the oscillatory nature of the calcium influx upon glucose stimulation. Our approach opens the doors to use the zebrafish as a model to investigate the contribution of genetic and environmental factors to beta-cell function and dysfunction.

Beta-cell functionality is important for blood-glucose homeostasis, which is evaluated at single-cell resolution using a genetically encoded reporter for calcium influx.

Análise da função de células Beta utilizando imagens de cálcio de célula única resolução em ilhotas de Zebrafish

Pancreatic beta-cells respond to increasing blood glucose concentrations by secreting the hormone insulin. The dysfunction of beta-cells leads to ...

Isolating Myofibrils from Skeletal Muscle Biopsies and Determining Contractile Function with a Nano-Newton Resolution Force Transducer

Striated muscle cells are indispensable for the activity of humans and animals. Single muscle fibers are comprised of myofibrils, which consist of serially linked sarcomeres, the smallest contractile units in muscle. Sarcomeric dysfunction contributes to muscle weakness in patients with mutations in genes encoding for sarcomeric proteins. The study of myofibril mechanics allows for the assessment of actin-myosin interactions without potential confounding effects of damaged, adjacent myofibrils when measuring the contractility of single muscle fibers. Ultrastructural damage and misalignment of myofibrils might contribute to impaired contractility. If structural damage is present in the myofibrils, they likely break during the isolation procedure or during the experiment. Furthermore, studies in myofibrils provide the assessment of actin-myosin interactions in the presence of the geometrical constraints of the sarcomeres. For instance, measurements in myofibrils can elucidate whether myofibrillar dysfunction is the primary effect of a mutation in a sarcomeric protein. In addition, perfusion with calcium solutions or compounds is almost instant due to the small diameter of the myofibril. This makes myofibrils eminently suitable to measure the rates of activation and relaxation during force production. The protocol described in this paper employs an optical force probe based on the principle of a Fabry-P&#233;rot interferometer capable of measuring forces in the nano-Newton range, coupled to a piezo length motor and a fast-step perfusion system. This setup enables the study of myofibril mechanics with high resolution force measurements.

Presented here is a protocol to assess the contractile properties of striated muscle myofibrils with nano-Newton resolution. The protocol employs a setup with an interferometry-based, optical force probe. This setup generates data with a high signal-to-noise ratio and enables the assessment of the contractile kinetics of myofibrils.