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The basic functional unit in a kidney is the nephron, which is a long and morphologically segmented tubule. The nephron begins with a cluster of capillaries called glomerulus through which the blood is filtered into the Bowman's space. The filtrate fl...
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RISS 인기검색어
Identification and classification of epithelial cells in nephron segments by actin cytoskeleton patterns
한글로보기https://www.riss.kr/link?id=O112923256
- 저자
- 발행기관
- 학술지명
- 권호사항
-
발행연도
2020년
-
작성언어
-
-
Print ISSN
1742-464X
-
Online ISSN
1742-4658
-
등재정보
SCI;SCIE;SCOPUS
-
자료형태
학술저널
-
수록면
1176-1194 [※수록면이 p5 이하이면, Review, Columns, Editor's Note, Abstract 등일 경우가 있습니다.]
-
구독기관
- 전북대학교 중앙도서관
- 성균관대학교 중앙학술정보관
- 부산대학교 중앙도서관
- 전남대학교 중앙도서관
- 제주대학교 중앙도서관
- 중앙대학교 서울캠퍼스 중앙도서관
- 인천대학교 학산도서관
- 숙명여자대학교 중앙도서관
- 서강대학교 로욜라중앙도서관
- 계명대학교 동산도서관
- 충남대학교 중앙도서관
- 한양대학교 백남학술정보관
- 이화여자대학교 중앙도서관
- 고려대학교 도서관
-
0
상세조회 -
0
다운로드
부가정보
다국어 초록 (Multilingual Abstract)
The basic functional unit in a kidney is the nephron, which is a long and morphologically segmented tubule. The nephron begins with a cluster of capillaries called glomerulus through which the blood is filtered into the Bowman's space. The filtrate flows through the nephron segments. During this flow, electrolytes and solutes are reabsorbed by channels and transport systems into the capillaries wrapped around the nephron. Many questions related to renal function focus on identifying the sites of expression of these systems. In this study, we mapped whole kidney sections by confocal microscopic imaging of fluorescent phalloidin, which binds to actin filaments. In tile scans (composed of hundreds of images) of these sections, the cortex and the medullary regions (outer and inner stripes of the outer medulla, and inner medulla) could be easily identified by their cytoskeletal patterns. At a higher resolution, we identified distinct features of the actin cytoskeleton in the apical, basal, and lateral borders of the cells. These features could be used to identify segments of a nephron (the proximal tubule, thin and thick segments of Henle's loop, and distal tubule), the collecting duct system, the papillary ducts in the papilla, and the urothelium that covers the pelvis. To verify our findings, we used additional markers, including aquaporin isoforms, cytokeratin 8‐18, and WGA lectin. This study highlights the power of high‐resolution confocal microscopy for identifying specific cell types using the simple probe of F‐actin‐binding phalloidin.
In this study, we mapped whole kidney sections by confocal microscopic imaging of fluorescent phalloidin that binds to actin filaments. At a high resolution, we identified actin cytoskeleton features of the apical, basal, and lateral borders of the epithelial cells to identify and distinguish between segments of a nephron (the proximal tubule, thin and thick segments of Henle's loop, and distal tubule) and the renal collecting duct system.
In this study, we mapped whole kidney sections by confocal microscopic imaging of fluorescent phalloidin that binds to actin filaments. At a high resolution, we identified actin cytoskeleton features of the apical, basal, and lateral borders of the epithelial cells to identify and distinguish between segments of a nephron (the proximal tubule, thin and thick segments of Henle's loop, and distal tubule) and the renal collecting duct system.
The basic functional unit in a kidney is the nephron, which is a long and morphologically segmented tubule. The nephron begins with a cluster of capillaries called glomerulus through which the blood is filtered into the Bowman's space. The filtrate flows through the nephron segments. During this flow, electrolytes and solutes are reabsorbed by channels and transport systems into the capillaries wrapped around the nephron. Many questions related to renal function focus on identifying the sites of expression of these systems. In this study, we mapped whole kidney sections by confocal microscopic imaging of fluorescent phalloidin, which binds to actin filaments. In tile scans (composed of hundreds of images) of these sections, the cortex and the medullary regions (outer and inner stripes of the outer medulla, and inner medulla) could be easily identified by their cytoskeletal patterns. At a higher resolution, we identified distinct features of the actin cytoskeleton in the apical, basal, and lateral borders of the cells. These features could be used to identify segments of a nephron (the proximal tubule, thin and thick segments of Henle's loop, and distal tubule), the collecting duct system, the papillary ducts in the papilla, and the urothelium that covers the pelvis. To verify our findings, we used additional markers, including aquaporin isoforms, cytokeratin 8‐18, and WGA lectin. This study highlights the power of high‐resolution confocal microscopy for identifying specific cell types using the simple probe of F‐actin‐binding phalloidin.
In this study, we mapped whole kidney sections by confocal microscopic imaging of fluorescent phalloidin that binds to actin filaments. At a high resolution, we identified actin cytoskeleton features of the apical, basal, and lateral borders of the epithelial cells to identify and distinguish between segments of a nephron (the proximal tubule, thin and thick segments of Henle's loop, and distal tubule) and the renal collecting duct system.
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