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Literature DB >> 8994823

Vital imaging: two photons are better than one.

Abstract

The recently developed technique of two-photon fluorescence microscopy causes much less photodamage than conventional confocal microscopy, expanding the possibilities for imaging living specimens.

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Year: 1996 PMID： 8994823 DOI： 10.1016/s0960-9822(02)70782-3

Source DB: PubMed Journal: Curr Biol ISSN： 0960-9822 Impact factor: 10.834

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Cited

15 in total

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Review 3. Use of reporter genes for optical measurements of neoplastic disease in vivo.

Authors: C H Contag; D Jenkins; P R Contag; R S Negrin
Journal: Neoplasia Date: 2000 Jan-Apr Impact factor: 5.715

Review 4. Trafficking of immune cells in the central nervous system.

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5. Hormonal regulation of nuclear permeability.

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6. Visualization of the distribution of autophosphorylated calcium/calmodulin-dependent protein kinase II after tetanic stimulation in the CA1 area of the hippocampus.

Authors: Y Ouyang; D Kantor; K M Harris; E M Schuman; M B Kennedy
Journal: J Neurosci Date: 1997-07-15 Impact factor: 6.167

7. Precisely timed spatiotemporal patterns of neural activity in dissociated cortical cultures.

Authors: J D Rolston; D A Wagenaar; S M Potter
Journal: Neuroscience Date: 2007-07-05 Impact factor: 3.590

8. Fast fluorescence microscopy for imaging the dynamics of embryonic development.

Authors: Julien Vermot; Scott E Fraser; Michael Liebling
Journal: HFSP J Date: 2008-05-13

9. MDL constrained 3-D grayscale skeletonization algorithm for automated extraction of dendrites and spines from fluorescence confocal images.

Authors: Xiaosong Yuan; Joshua T Trachtenberg; Steve M Potter; Badrinath Roysam
Journal: Neuroinformatics Date: 2009-12-11

Review 10. The fluorescent protein palette: tools for cellular imaging.

Authors: Richard N Day; Michael W Davidson
Journal: Chem Soc Rev Date: 2009-08-04 Impact factor: 54.564