Metabolomic approach for identifying and visualizing molecular tissue markers in tadpoles of <i>Xenopus tropicalis</i> by mass spectrometry imaging

Goto‐Inoue, Naoko; Kashiwagi, Akihiko; Kashiwagi, Kazuhiro; Mori, Tsukasa

doi:10.1242/bio.019646

Cited by 17 publications

(16 citation statements)

References 31 publications

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“…The serial sections were mounted onto glass slides (Matsunami, Osaka, Japan) for hemotoxylin and eosin (H&E) staining and immunofluorescence staining and onto indium tin oxide (ITO)‐coated glass slides (Bruker Daltonics, Germany) for MSI. Samples were prepared according to a previously published method . Briefly, appropriate matrix solutions, including 50 mg/mL DHB in methanol/water (8:2, v/v) for positive ion mode and 20 mg/mL 9‐AA in ethanol/water (8:2, v/v) for negative ion mode, were used.…”

Section: Methodsmentioning

confidence: 99%

Characterization of myofiber‐type‐specific molecules using mass spectrometry imaging

Goto‐Inoue

Morisasa

Machida

et al. 2018

Rapid Comm Mass Spectrometry

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Rationale:In skeletal muscles, there are four myofiber types, Types I, IIa, IIx, and IIb, which show different contraction characteristics and have different metabolic statuses. To understand muscle function, it is necessary to analyze myofiber-specific metabolic changes. However, these fibers are heterogeneous and are hard to discriminate by conventional analyses using tissue extracts. In this study, we found myofiber-specific molecules and molecular markers of other cells such as smooth muscle cells, fat cells, and motor neurons, and visualized them within muscle sections. Methods:We used three different muscle tissues, namely extensor digitorum longus, soleus, and gastrocnemius tissues, from ICR mice. After the muscles had been harvested, cross-sections were prepared using a cryostat and analyzed using matrixassisted laser desorption/ionization (MALDI) mass spectrometry imaging (MSI), and conventional immunofluorescence imaging.Results: By comparing the MALDI MSI results with the immunofluorescence imaging results, we were able to identify each fiber and cell-specific ion. It was especially important that we could find Type IIa and IIb specific ions, because these were difficult to distinguish. Conclusions:Through MSI analyses, we performed a comprehensive survey to identify cell-and myofiber-specific molecular markers. In conclusion, we assigned muscle fiber Type I, IIa, and IIb-specific molecular ions at m/z 856.6, 872.6, and 683.8, respectively. These molecular markers might be useful for verifying changes that occur due to exercise and/or disease.

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Section: Methodsmentioning

confidence: 99%

Characterization of myofiber‐type‐specific molecules using mass spectrometry imaging

Goto‐Inoue

Morisasa

Machida

et al. 2018

Rapid Comm Mass Spectrometry

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“…After MS imaging, the sections were also subjected to HE staining for morphological observation. Samples were prepared as described previously 26,27 . Briefly, a matrix solution containing 50 mg/mL 2,5-dihydroxybenzoic acid in methanol:water (8:2, v/v) was used, with 1-2 mL of it prepared before use and sprayed uniformly over the frozen sections using an airbrush with a 0.2-mm nozzle (Procon Boy FWA Platinum; Mr. Hobby, Tokyo, Japan).…”

Section: Methodsmentioning

confidence: 99%

Mass spectrometry imaging reveals differential localization of natural sunscreens in the mantle of the giant clam Tridacna crocea

Goto‐Inoue

Satō

Morisasa

et al. 2020

Sci Rep

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Giant clams have evolved to maximize sunlight utilization by their photosymbiotic partners, while affording them protection from harmful ultraviolet (UV) light. The presence of UV absorbing substances in the mantle is thought to be critical for light protection; however, the exact localization of such compounds remains unknown. Here, we applied a combination of UV liquid chromatography (LC), LC-mass spectrometry (MS), MS imaging, and UV micrography to localize UV absorbing substances in the giant clam Tridacna crocea. LC-MS analysis revealed that the animal contained three classes of mycosporines: progenitor, primary, and secondary mycosporines. MS imaging revealed that primary and secondary mycosporines were localized in the outermost layer of the mantle; whereas progenitor mycosporines were distributed throughout the mantle tissue. These findings were consistent with the results of UV micrography, which revealed that the surface layer of the mantle absorbed UV light at 320 ± 10 nm. This is the first report indicating that progenitor and primary mycosporines are metabolized to secondary mycosporines by the giant clam and that they are differentially localized in the surface layer of the mantle to protect the animal from UV light.

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“…11 Tadpoles were then bred for 10 days and harvested using cryopreservation as described. 12 Briefly, tadpoles without tails were freeze embedded in blocks with 4%…”

Section: Preparation Of Tissue Sectionsmentioning

confidence: 99%

Novel approach to enhance sensitivity while retaining morphology in fragile tissue sections for mass spectrometry imaging

et al. 2020

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Matrix‐assisted laser desorption/ionization mass spectrometry (MALDI‐MS) imaging is an effective tool for investigating the distribution of molecules. However, cryosections are made from non‐fixed tissues, causing difficulties in preparing sections from fragile, high‐water content tissues such as those from tadpoles. Here, we introduce a new method for preparing cryosections using an adhesive tape followed by transfer onto glass slides for MALDI‐MS imaging. Signals obtained from the transferred sections were higher than those from other sections, and the transferred sections had high optical quality. This novel approach could be an effective tool for MALDI‐MS imaging of aquatic animals.

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Metabolomic approach for identifying and visualizing molecular tissue markers in tadpoles of Xenopus tropicalis by mass spectrometry imaging

Cited by 17 publications

References 31 publications

Characterization of myofiber‐type‐specific molecules using mass spectrometry imaging

Characterization of myofiber‐type‐specific molecules using mass spectrometry imaging

Mass spectrometry imaging reveals differential localization of natural sunscreens in the mantle of the giant clam Tridacna crocea

Novel approach to enhance sensitivity while retaining morphology in fragile tissue sections for mass spectrometry imaging

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