MicroMagnify: A Multiplexed Expansion Microscopy Method for Pathogens and Infected Tissues

Cheng, Zhangyu; Stefani, Caroline; Skillman, Thomas; Klimas, Aleksandra; Lee, Aramchan; DiBernardo, Emma F.; Brown, Karina Mueller; Milman, Tatyana; Wang, Yuhong; Gallagher, Brendan R.; Lagree, Katherine; Jena, Bhanu P.; Pulido, Jose S.; Filler, Scott G.; Mitchell, Aaron P.; Hiller, N. Luisa; Lacy‐Hulbert, Adam; Zhao, Yongxin

doi:10.1002/advs.202302249

Cited by 9 publications

(4 citation statements)

References 49 publications

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“…In the few years since its invention, ExM has already shown remarkable compatibility with super-resolution microscopy approaches and various ‘omics’ techniques, and has been tested in a wide variety of species and even samples from patients. ExM protocols that allow the processing of formalin-fixed, paraffin-embedded tissue samples have been essential in allowing this progress ( Bai et al, 2023 ; Mao et al, 2020 ; Unnersjö-Jess et al, 2022 ; Zhao et al, 2017 ; Cheng et al, 2023 ). If such sample preparation protocols can be implemented in high-throughput automation and imaging, ExM has the potential to also have a high impact on diagnostics.…”

Section: Discussionmentioning

confidence: 99%

Expanding boundaries – a cell biologist's guide to expansion microscopy

Hümpfer,

Thielhorn,

Ewers

2024

Journal of Cell Science

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Expansion microscopy (ExM) is a revolutionary novel approach to increase resolution in light microscopy. In contrast to super-resolution microscopy methods that rely on sophisticated technological advances, including novel instrumentation, ExM instead is entirely based on sample preparation. In ExM, labeled target molecules in fixed cells are anchored in a hydrogel, which is then physically enlarged by osmotic swelling. The isotropic swelling of the hydrogel pulls the labels apart from one another, and their relative organization can thus be resolved using conventional microscopes even if it was below the diffraction limit of light beforehand. As ExM can additionally benefit from the technical resolution enhancements achieved by super-resolution microscopy, it can reach into the nanometer range of resolution with an astoundingly low degree of error induced by distortion during the physical expansion process. Because the underlying chemistry is well understood and the technique is based on a relatively simple procedure, ExM is easily reproducible in non-expert laboratories and has quickly been adopted to address an ever-expanding spectrum of problems across the life sciences. In this Review, we provide an overview of this rapidly expanding new field, summarize the most important insights gained so far and attempt to offer an outlook on future developments.

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Section: Discussionmentioning

confidence: 99%

Expanding boundaries – a cell biologist's guide to expansion microscopy

Hümpfer,

Thielhorn,

Ewers

2024

Journal of Cell Science

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“…Importantly, it eliminates the need for access to costly super-resolution microscopes to achieve sub diffraction-resolution fluorescence imaging of cellular structures. Although expansion microscopy was only recently established as a new imaging modality, several protocols have now been developed for expanding cells and tissues from a variety of organisms including bacteria, parasites, insects and vertebrates (Atchou et al, 2023; Bai et al, 2023; Bandeira et al, 2023; Campbell et al, 2021; Chang et al, 2024; Chang et al, 2017; Chen et al, 2015; Cheng et al, 2023; Ching et al, 2022; Chozinski et al, 2016; Chozinski et al, 2018; Damstra et al, 2022; Damstra et al, 2023; Dos Santos Pacheco & Soldati-Favre, 2021; Fan et al, 2021; Gallagher & Zhao, 2021; Gambarotto et al, 2021; Gambarotto et al, 2019; Gaudreau-Lapierre et al, 2021; Hamel & Guichard, 2021; Jurriens et al, 2021; Klimas et al, 2023; Kraft et al, 2023; Ku et al, 2016; Kunz et al, 2019; Kunz et al, 2021; Liffner et al, 2023; Lin et al, 2022; Louvel et al, 2023; Mäntylä et al, 2023; Middelhauve et al, 2023; Moye et al, 2023; Murakami et al, 2018; Park et al, 2019; Park et al, 2021; Parveen et al, 2023; Perelsman et al, 2022; Pernal et al, 2020; Pesce et al, 2019; Ponjavić et al, 2021; Rodriguez-Gatica et al, 2022; Sahabandu et al, 2019; Siegerist et al, 2022; Steib et al, 2022; Tillberg & Chen, 2019; Tillberg et al, 2016; Unnersjö-Jess et al, 2021; Unnersjö-Jess et al, 2018; Wainman, 2021; Wang et al, 2018; Wassie et al, 2019; Wen et al, 2023; Wilmerding et al, 2023; Woo et al, 2020; Yu et al, 2022; Zhao et al, 2017; Zhu et al, 2021; Zhuang & Shi, 2024).…”

Section: Introductionmentioning

confidence: 99%

Ultrastructure expansion microscopy (U-ExM) of mouse and human kidneys for analysis of subcellular structures

Langner,

Puapatanakul,

Pudlowski

et al. 2024

Preprint

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Ultrastructure expansion microscopy (U-ExM) involves the physical magnification of specimens embedded in hydrogels, which allows for super-resolution imaging of subcellular structures using a conventional diffraction-limited microscope. Methods for expansion microscopy exist for several organisms, organs, and cell types, and used to analyze cellular organelles and substructures in nanoscale resolution. Here, we describe a simple step-by-step U-ExM protocol for the expansion, immunostaining, imaging, and analysis of cytoskeletal and organellar structures in kidney tissue. We detail the critical modified steps to optimize isotropic kidney tissue expansion, and preservation of the renal cell structures of interest. We demonstrate the utility of the approach using several markers of renal cell types, centrioles, cilia, the extracellular matrix, and other cytoskeletal elements. Finally, we show that the approach works well on mouse and human kidney samples that were preserved using different fixation and storage conditions. Overall, this protocol provides a simple and cost-effective approach to analyze both pre-clinical and clinical renal samples in high detail, using conventional lab supplies and standard widefield or confocal microscopy.

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“…8,9 So, the rapid and accurate diagnosis of infectious diseases is crucial. 10 The identification of microorganisms can effectively identify the types of pathogens and guide the right treatment. Traditional methods for bacterial analysis, for example, the plate counting method, polymerase chain reaction (PCR), enzyme-linked immunosorbent assay (ELISA), and mass spectrometry, are well-established but often labor-intensive and operationally complex.…”

mentioning

confidence: 99%

“…Notably, bacterial infections are highlighted by the World Health Organization as the top 10 threats to global health . Although antibiotics are effective in treating bacteria and fungi, long-term abuse of antibiotics causes strains to mutate, resulting in antibiotic resistance. , So, the rapid and accurate diagnosis of infectious diseases is crucial . The identification of microorganisms can effectively identify the types of pathogens and guide the right treatment.…”

mentioning

confidence: 99%

Identification of Microorganism in Infected Wounds by Positively Charged Selective Sensor Array and Deep Learning Algorithm

Zhang,

Ma,

Wang

et al. 2024

Anal. Chem.

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Microorganism are ubiquitous and intimately connected with human health and disease management. The accurate and fast identification of pathogenic microorganisms is especially important for diagnosing infections. Herein, three tetraphenylethylene derivatives (S-TDs: TBN, TPN, and TPI) featuring different cationic groups, charge numbers, emission wavelengths, and hydrophobicities were successfully synthesized. Benefiting from distinct cell wall binding properties, S-TDs were collectively utilized to create a sensor array capable of imaging various microorganisms through their characteristic fluorescent signatures. Furthermore, the interaction mechanism between S-TDs and different microorganisms was explored by calculating the binding energy between S-TDs and cell membrane/wall constituents, including phospholipid bilayer and peptidoglycan. Using a combination of the fluorescence sensor array and a deep learning model of residual network (ResNet), readily differentiation of Gram-negative bacteria (G−), Gram-positive bacteria (G+), fungi, and their mixtures was achieved. Specifically, by extensive training of two ResNet models with large quantities of images data from 14 kinds of microorganism stained with S-TDs, identification of microorganism was achieved at high-level accuracy: over 92.8% for both Gram species and antibiotic-resistant species, with 90.35% accuracy for the detection of mixed microorganism in infected wound. This novel method provides a rapid and accurate method for microbial classification, potentially aiding in the diagnosis and treatment of infectious diseases.

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MicroMagnify: A Multiplexed Expansion Microscopy Method for Pathogens and Infected Tissues

Cited by 9 publications

References 49 publications

Expanding boundaries – a cell biologist's guide to expansion microscopy

Expanding boundaries – a cell biologist's guide to expansion microscopy

Ultrastructure expansion microscopy (U-ExM) of mouse and human kidneys for analysis of subcellular structures

Identification of Microorganism in Infected Wounds by Positively Charged Selective Sensor Array and Deep Learning Algorithm

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