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분자분광학및동력학연구단
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Label-free neuroimaging in vivo using synchronous angular scanning microscopy with single-scattering accumulation algorithm

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dc.contributor.authorMoonseok Kim-
dc.contributor.authorYonghyeon Jo-
dc.contributor.authorJin Hee Hong-
dc.contributor.authorKim, Suhyun-
dc.contributor.authorSeokchan Yoon-
dc.contributor.authorKyung-Deok Song-
dc.contributor.authorKang, Sungsam-
dc.contributor.authorLee, Byunghak-
dc.contributor.authorKim, Guang Hoon-
dc.contributor.authorPark, Hae-Chul-
dc.contributor.authorWonshik Choi-
dc.date.available2019-09-25T07:24:25Z-
dc.date.created2019-08-20-
dc.date.issued2019-07-
dc.identifier.issn2041-1723-
dc.identifier.urihttps://pr.ibs.re.kr/handle/8788114/6132-
dc.description.abstract© 2019, The Author(s).Label-free in vivo imaging is crucial for elucidating the underlying mechanisms of many important biological systems in their most native states. However, the applicability of existing modalities has been limited to either superficial layers or early developmental stages due to tissue turbidity. Here, we report a synchronous angular scanning microscope for the rapid interferometric recording of the time-gated reflection matrix, which is a unique matrix characterizing full light-specimen interaction. By applying single scattering accumulation algorithm to the recorded matrix, we removed both high-order sample-induced aberrations and multiple scattering noise with the effective aberration correction speed of 10,000 modes/s. We demonstrated in vivo imaging of whole neural network throughout the hindbrain of the larval zebrafish at a matured stage where physical dissection used to be required for conventional imaging. Our method will expand the scope of applications for optical imaging, where fully non-invasive interrogation of living specimens is critical-
dc.description.uri1-
dc.language영어-
dc.publisherNATURE PUBLISHING GROUP-
dc.subjectAdaptive optics, Image processing, Interference microscopy, Optical imaging-
dc.titleLabel-free neuroimaging in vivo using synchronous angular scanning microscopy with single-scattering accumulation algorithm-
dc.typeArticle-
dc.type.rimsART-
dc.identifier.wosid000475833800001-
dc.identifier.scopusid2-s2.0-85069441913-
dc.identifier.rimsid69315-
dc.contributor.affiliatedAuthorMoonseok Kim-
dc.contributor.affiliatedAuthorYonghyeon Jo-
dc.contributor.affiliatedAuthorJin Hee Hong-
dc.contributor.affiliatedAuthorSeokchan Yoon-
dc.contributor.affiliatedAuthorKyung-Deok Song-
dc.contributor.affiliatedAuthorWonshik Choi-
dc.identifier.doi10.1038/s41467-019-11040-z-
dc.identifier.bibliographicCitationNATURE COMMUNICATIONS, v.10, no.1, pp.3152-
dc.citation.titleNATURE COMMUNICATIONS-
dc.citation.volume10-
dc.citation.number1-
dc.citation.startPage3152-
dc.description.journalClass1-
dc.description.journalRegisteredClassscie-
dc.description.journalRegisteredClassscopus-
dc.subject.keywordPlusADAPTIVE OPTICS-
dc.subject.keywordPlusABERRATION CORRECTION-
dc.subject.keywordPlusRESOLUTION-
dc.subject.keywordPlusDEEP-
dc.subject.keywordPlusMYELINATION-
dc.subject.keywordPlusTOMOGRAPHY-
dc.subject.keywordPlusNEURONS-
Appears in Collections:
Center for Molecular Spectroscopy and Dynamics(분자 분광학 및 동력학 연구단) > 1. Journal Papers (저널논문)
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