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1. Comparative analysis of the transcriptomes of EDL, psoas, and soleus muscles from mice

   https://doi.org/10.1186/s12864-020-07225-2  

   Hettige, Pabodha; Tahir, Uzma; Nishikawa, Kiisa C.; Gage, Matthew J. (December 2020, BMC Genomics)

   null (Ed.)

   Abstract Background Individual skeletal muscles have evolved to perform specific tasks based on their molecular composition. In general, muscle fibers are characterized as either fast-twitch or slow-twitch based on their myosin heavy chain isoform profiles. This approach made sense in the early days of muscle studies when SDS-PAGE was the primary tool for mapping fiber type. However, Next Generation Sequencing tools permit analysis of the entire muscle transcriptome in a single sample, which allows for more precise characterization of differences among fiber types, including distinguishing between different isoforms of specific proteins. We demonstrate the power of this approach by comparing the differential gene expression patterns of extensor digitorum longus (EDL), psoas, and soleus from mice using high throughput RNA sequencing. Results EDL and psoas are typically classified as fast-twitch muscles based on their myosin expression pattern, while soleus is considered a slow-twitch muscle. The majority of the transcriptomic variability aligns with the fast-twitch and slow-twitch characterization. However, psoas and EDL exhibit unique expression patterns associated with the genes coding for extracellular matrix, myofibril, transcription, translation, striated muscle adaptation, mitochondrion distribution, and metabolism. Furthermore, significant expression differences between psoas and EDL were observed in genes coding for myosin light chain, troponin, tropomyosin isoforms, and several genes encoding the constituents of the Z-disk. Conclusions The observations highlight the intricate molecular nature of skeletal muscles and demonstrate the importance of utilizing transcriptomic information as a tool for skeletal muscle characterization. 

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2. Continuous Viscoelasticity Measurement of Cell Spheroids via Microfluidic Electrical Aspiration

   https://doi.org/10.1021/acssensors.4c01405  

   Chen, Heyi; Brown, Jacob; Urban, Aaron; Zhang, Ge; Zhe, Jiang (November 2024, ACS Sensors)

   Measurement of viscoelastic characteristics of cells cultured in 3D is critical to study many biological processes including tissue and organ growth. In this article, we present a unique electrical aspiration method to measure the viscoelastic properties of cell spheroids. A microfluidic sensor was created to demonstrate this method. Unlike the traditional optical aspiration method, the aspiration of the cell spheroids is monitored via monitoring the dynamic electrical resistance change of a symmetrical microfluidic aspiration channel. We first used the microfluidic device to measure the viscoelastic properties of two types of biological tissues derived from calfskin and porcine left ventricular myocardium. The equilibrium elastic modulus and creep time con-stants were measured to be 148.1±24.1 kPa and 76.7±3.5seconds and 64.5±7.7 kPa and 31.4±2.7 seconds respectively, which matched well with reported data. The test validated the principle of the electrical aspiration method. Next, we applied the method for measuring cell spheroids made of human mesenchymal stem cells at different culture stages. The equilibrium elastic modulus and apparent viscosity decreased with increasing culture time. Compared to optical aspiration methods, this microfluidic electrical aspiration method has no reliance on transparent materials and image processing, which thus allows simple set-up, fast data acquisition and analysis. The use of a symmetric aspiration channel and the linear half-space model enable measurements of a large number of viscoelastic properties via a single measurement with higher accuracy. This method will enable high throughput, continuous viscoelastic measurement of cell spheroids as well as other 3D cell culture models in flow conditions without the need for any optical measurements 

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3. Variations in Tissue Interactions During Head Muscle Development

   https://doi.org/10.1002/ar.25522  

   Ziermann-Canabarro, Janine M; Correa-Alfonzo, Paola (June 2024, The Anatomical Record)

   For decades it has been established that head muscle development differs from trunk muscle development. Similarly known, even though not in such detail, is that different subgroups of head muscles develop dependent on different underlying gene regulatory networks. Even less well studied are the tissue interactions during the developmental processes. Muscles derived from pharyngeal arch mesoderm depend on interactions with endoderm and neural crest cells, and, to a minor extent, ectodermal cues. Extraocular eye muscles respond to a mix of signals from surrounding mesoderm, but also neural crest cells; however, they are independent of endodermal cues. Head muscles derived from occipital paraxial mesoderm depend on tissue interactions similar to pharyngeal arch muscles but have a different migration trajectory. While the pharyngeal arch mesodermal cells and neural crest cells largely migrate from dorsal to ventral, the occipital paraxial mesodermal cells migrate from dorsal to ventral and from posterior to anterior. During the migration these cells proliferate and even start to differentiate, while pharyngeal mesodermal cells begin the differentiation process after reaching their respective pharyngeal arches. Here we present an overview of tissue interactions during the development of different head muscle populations, highlighting general concepts and main differences. Topic Category: Neural Crest, Placodes and Craniofacial Development Keywords: Craniofacial muscles, Myogenesis Funding or Support Information: NSF #2000005 to JMZC 

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4. Towards a standardized multi-tissue decellularization protocol for the derivation of extracellular matrix materials

   https://doi.org/10.1039/d2bm01012g  

   Biehl, Andreea; Gracioso Martins, Ana M.; Davis, Zachary G.; Sze, Daphne; Collins, Leonard; Mora-Navarro, Camilo; Fisher, Matthew B.; Freytes, Donald O. (January 2023, Biomaterials Science)

   The goal of tissue decellularization is to efficiently remove unwanted cellular components, such as DNA and cellular debris, while retaining the complex structural and molecular milieu within the extracellular matrix (ECM). Decellularization protocols to date are centered on customized tissue-specific and lab-specific protocols that involve consecutive manual steps which results in variable and protocol-specific ECM material. The differences that result from the inconsistent protocols between decellularized ECMs affect consistency across batches, limit comparisons between results obtained from different laboratories, and could limit the transferability of the material for consistent laboratory or clinical use. The present study is the first proof-of-concept towards the development of a standardized protocol that can be used to derive multiple ECM biomaterials (powders and hydrogels) via a previously established automated system. The automated decellularization method developed by our group was used due to its short decellularization time (4 hours) and its ability to reduce batch-to-batch variability. The ECM obtained using this first iteration of a unified protocol was able to produce ECM hydrogels from skin, lung, muscle, tendons, cartilage, and laryngeal tissues. All hydrogels formed in this study were cytocompatible and showed gelation and rheological properties consistent with previous ECM hydrogels. The ECMs also showed unique proteomic composition. The present study represents the first step towards developing standardized protocols that can be used on multiple tissues in a fast, scalable, and reproducible manner. 

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5. Proteomic and Bioinformatic Analysis of Decellularized Pancreatic Extracellular Matrices

   https://doi.org/10.3390/molecules26216740  

   Hu, Ming; Bi, Huanjing; Moffat, Deana; Blystone, Margaret; DeCostanza, Paul; Alayi, Tchilabalo; Ye, Kaiming; Hathout, Yetrib; Jin, Sha (November 2021, Molecules)

   Tissue microenvironments are rich in signaling molecules. However, factors in the tissue matrix that can serve as tissue-specific cues for engineering pancreatic tissues have not been thoroughly identified. In this study, we performed a comprehensive proteomic analysis of porcine decellularized pancreatic extracellular matrix (dpECM). By profiling dpECM collected from subjects of different ages and genders, we showed that the detergent-free decellularization method developed in this study permits the preservation of approximately 62.4% more proteins than a detergent-based method. In addition, we demonstrated that dpECM prepared from young pigs contained approximately 68.5% more extracellular matrix proteins than those prepared from adult pigs. Furthermore, we categorized dpECM proteins by biological process, molecular function, and cellular component through gene ontology analysis. Our study results also suggested that the protein composition of dpECM is significantly different between male and female animals while a KEGG enrichment pathway analysis revealed that dpECM protein profiling varies significantly depending on age. This study provides the proteome of pancreatic decellularized ECM in different animal ages and genders, which will help identify the bioactive molecules that are pivotal in creating tissue-specific cues for engineering tissues in vitro. 

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