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	<title>Bench Marks &#187; Imaging&#047;Microscopy</title>
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		<title>Bench Marks &#187; Imaging&#047;Microscopy</title>
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		<title>3D Imaging of Embryos is Featured in CSH Protocols</title>
		<link>http://cshbenchmarks.wordpress.com/2011/06/01/opt/</link>
		<comments>http://cshbenchmarks.wordpress.com/2011/06/01/opt/#comments</comments>
		<pubDate>Wed, 01 Jun 2011 14:28:27 +0000</pubDate>
		<dc:creator>Bench Marks</dc:creator>
				<category><![CDATA[Developmental Biology]]></category>
		<category><![CDATA[Imaging/Microscopy]]></category>

		<guid isPermaLink="false">http://cshbenchmarks.wordpress.com/?p=2076</guid>
		<description><![CDATA[Until recently, a common technique for creating a 3D image of an embryo was to slice it into hundreds of thin sections, photograph each section, and then computationally recombine the images to produce a 3D representation of the embryo.  But during this process, the specimen may become deformed, and information about the alignment of the [...]<img alt="" border="0" src="http://stats.wordpress.com/b.gif?host=cshbenchmarks.wordpress.com&amp;blog=20090526&amp;post=2076&amp;subd=cshbenchmarks&amp;ref=&amp;feed=1" width="1" height="1" />]]></description>
			<content:encoded><![CDATA[<p style="text-align:justify;"><img class="alignleft size-full wp-image-2078" title="3D imaging of vertebrate development by OPT" src="http://cshbenchmarks.files.wordpress.com/2011/06/opt.jpg?w=510" alt=""   />Until recently, a common technique for creating a 3D image of an embryo was to slice it into hundreds of thin sections, photograph each section, and then computationally recombine the images to produce a 3D representation of the embryo.  But during this process, the specimen may become deformed, and information about the alignment of the sections – the third dimension – is lost.</p>
<p style="text-align:justify;">Optical projection tomography (OPT) overcomes these problems, as <a href="http://pasteur.crg.es/portal/page/portal/Internet/02_Research/01_Programmes/06_Systems_Biology/03_Systems_Analysis_of_Development">Laura Quintana and James Sharpe (Centre for Genomic Regulation, Barcelona)</a> explain in <a href="http://cshprotocols.cshlp.org/cgi/content/full/2011/6/pdb.top116">a featured article</a> in the latest issue of <em>Cold Spring Harbor Protocols</em>.  OPT is ideal for analyzing the morphology of fixed embryos – especially for analyzing mutant phenotypes, for developing anatomical atlases, and for analyzing gene expression patterns. <span id="more-2076"></span></p>
<p style="text-align:justify;">During OPT, the whole embryo is mounted on a stage that rotates 360 degrees.  As the embryo rotates, visible light is projected through it, and a detector on the other side records the amount of light that penetrates.  Images are captured at different angles as it revolves, and computer software combines the images to create a 3D image.</p>
<p style="text-align:justify;">Sharpe, the lead author of the article, describes OPT in this video:</p>
<p style="text-align:justify;"><span style="text-align:center; display: block;"><a href="http://cshbenchmarks.wordpress.com/2011/06/01/opt/"><img src="http://img.youtube.com/vi/CwXw7Jx-_eU/2.jpg" alt="" /></a></span></p>
<p style="text-align:justify;">The article, freely accessible <a href="http://cshprotocols.cshlp.org/cgi/content/full/2011/6/pdb.top116">here</a>, is published in the June issue.  The issue also contains <a href="http://cshprotocols.cshlp.org/cgi/content/full/2011/6/pdb.prot5639">a detailed step-by-step protocol</a>, written by the same authors, for the preparation of mouse embryos for OPT imaging.</p>
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			<media:title type="html">mariasmit</media:title>
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			<media:title type="html">3D imaging of vertebrate development by OPT</media:title>
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		<title>CSH Protocols Features Methods for Imaging Kidney Development</title>
		<link>http://cshbenchmarks.wordpress.com/2011/05/02/csh-protocols-features-methods-for-imaging-kidney-development/</link>
		<comments>http://cshbenchmarks.wordpress.com/2011/05/02/csh-protocols-features-methods-for-imaging-kidney-development/#comments</comments>
		<pubDate>Mon, 02 May 2011 20:11:00 +0000</pubDate>
		<dc:creator>Bench Marks</dc:creator>
				<category><![CDATA[Developmental Biology]]></category>
		<category><![CDATA[Imaging/Microscopy]]></category>

		<guid isPermaLink="false">http://cshbenchmarks.wordpress.com/?p=1988</guid>
		<description><![CDATA[The adult mouse kidney begins to develop at embryonic day 10.5, when the epithelial ureteric bud evaginates from the Wolffian duct and grows into adjacent metanephric mesenchyme.  Over the course of several days, the ureteric bud repeatedly branches, giving rise to the ureter, pelvis, calyces, and renal collecting ducts of the adult kidney. The kidney [...]<img alt="" border="0" src="http://stats.wordpress.com/b.gif?host=cshbenchmarks.wordpress.com&amp;blog=20090526&amp;post=1988&amp;subd=cshbenchmarks&amp;ref=&amp;feed=1" width="1" height="1" />]]></description>
			<content:encoded><![CDATA[<p style="text-align:justify;"><a href="http://cshprotocols.cshlp.org/TOCs/toc5_11.dtl"><img class="alignleft size-thumbnail wp-image-1989" title="CSH Protocols, May 2011" src="http://cshbenchmarks.files.wordpress.com/2011/05/05_2011_cover.jpg?w=116&#038;h=150" alt="CSH Protocols, May 2011" width="116" height="150" /></a>The adult mouse kidney begins to develop at embryonic day 10.5, when the epithelial ureteric bud evaginates from the Wolffian duct and grows into adjacent metanephric mesenchyme.  Over the course of several days, the ureteric bud repeatedly branches, giving rise to the ureter, pelvis, calyces, and renal collecting ducts of the adult kidney.</p>
<p style="text-align:justify;">The kidney can develop in culture, from the first stage of ureteric bud evagination through the first 8-10 rounds of branching.  These processes can therefore be visualized through time-lapse imaging, providing a greater understanding of normal kidney morphogenesis and how genetic perturbations affect kidney development.</p>
<p style="text-align:justify;">This month’s issue of <em>Cold Spring Harbor Protocols</em>, out today, features <a href="http://cshprotocols.cshlp.org/cgi/content/full/2011/5/pdb.top109">an article that presents the general concepts of imaging kidney development</a> and describes genetically modified mice that express fluorescent proteins useful for visualizing different cell lineages and developmental processes in these organ cultures.  <a href="http://cshprotocols.cshlp.org/cgi/content/abstract/2011/5/pdb.prot5613">A detailed step-by-step protocol for dissecting, culturing, and imaging embryonic mouse kidneys</a> is also published in the issue.  Both articles were written by <a href="http://asp.cumc.columbia.edu/facdb/profile_list.asp?uni=fdc3&amp;DepAffil=Genetics">Frank Costantini (Columbia University Medical Center)</a>, <a href="http://www.dpag.ox.ac.uk/academic_staff/shankar_srinivas">Shankar Srinivas (University of Oxford)</a>, and colleagues.</p>
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			<media:title type="html">mariasmit</media:title>
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			<media:title type="html">CSH Protocols, May 2011</media:title>
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		<title>Neuroscience Tools with Extraordinary Precision:  Quantum Dots and Microbial Opsins</title>
		<link>http://cshbenchmarks.wordpress.com/2011/03/07/neuroscience-tools-with-extraordinary-precision-quantum-dots-and-microbial-opsins/</link>
		<comments>http://cshbenchmarks.wordpress.com/2011/03/07/neuroscience-tools-with-extraordinary-precision-quantum-dots-and-microbial-opsins/#comments</comments>
		<pubDate>Mon, 07 Mar 2011 14:49:59 +0000</pubDate>
		<dc:creator>Bench Marks</dc:creator>
				<category><![CDATA[Imaging/Microscopy]]></category>
		<category><![CDATA[Neuroscience]]></category>

		<guid isPermaLink="false">http://cshbenchmarks.wordpress.com/?p=1785</guid>
		<description><![CDATA[As a preview to the forthcoming laboratory manual Imaging in Neuroscience, due in May, the current issue of Cold Spring Harbor Protocols highlights two articles on neuroscience imaging techniques.  The articles are freely accessible here and here. Monitoring Individual Molecules with Quantum Dots The first article details the use of nanometer-sized quantum dots (QDs) to [...]<img alt="" border="0" src="http://stats.wordpress.com/b.gif?host=cshbenchmarks.wordpress.com&amp;blog=20090526&amp;post=1785&amp;subd=cshbenchmarks&amp;ref=&amp;feed=1" width="1" height="1" />]]></description>
			<content:encoded><![CDATA[<p>As a preview to the forthcoming laboratory manual <a href="http://www.cshlpress.com/link/imagingneurop.htm"><em>Imaging in Neuroscience</em></a>, due in May, the current issue of <a href="http://cshprotocols.cshlp.org/"><em>Cold Spring Harbor Protocols</em></a> highlights two articles on neuroscience imaging techniques.  The articles are freely accessible <a href="http://cshprotocols.cshlp.org/cgi/content/full/2011/3/prot5580">here</a> and <a href="http://cshprotocols.cshlp.org/cgi/content/full/2011/3/top102">here</a>.</p>
<p><strong>Monitoring Individual Molecules with Quantum Dots</strong></p>
<p><a href="http://cshprotocols.cshlp.org/cgi/content/full/2011/3/prot5580">The first article</a> details the use of nanometer-sized quantum dots (QDs) to track the motion of individual membrane molecules over time.  QDs possess strong fluorescence and photostability, permitting extended recording times compared to other methods.  In the article, authors Sabine Lévi, Maxime Dahan, and Antoine Triller (Ecole Normale Supérieure, Paris) provide step-by-step methods to stain neurons with QDs and to track QD-labeled molecules using single-fluorophore epifluorescence, as well as guidance for interpreting the data and reconstructing the trajectory of individual QD-labeled molecules.  These methods have been successfully used to follow the diffusion of individual glycine receptors, GABA receptors, NMDA receptors, lipid raft markers, glycophosphatidylinositol-anchored green fluorescent protein (GPI-GFP), and other molecules of interest.</p>
<p><strong>Studying Specific Neural Activities with Microbial Opsins</strong></p>
<p><a href="http://cshprotocols.cshlp.org/cgi/content/full/2011/3/top102">The second article</a> describes characteristics of various microbial opsins that are used in optogenetics.  Optogenetics is a revolutionary technology that combines optics and genetics to study very specific events, such as action potentials, in their natural context—even in freely moving mammals.  Microbial opsins are light-sensing proteins that regulate ion fluxes to control biological activities, and their corresponding genes can be expressed in mammalian neurons to enable millisecond-precision optical control of neural activity.  The authors of the article, <a href="http://www.stanford.edu/group/dlab/">Karl Diesseroth and colleagues (Stanford)</a> and <a href="http://www2.hu-berlin.de/biologie/expbp/">Peter Hegemann (Humboldt-Universität, Berlin)</a>, describe the diversity of microbial opsin genes, including those for bacteriorhodopsins, proteorhodopsins, halorhodopsins, and channelrhodopsins, and the structure-function properties of their corresponding proteins.  This overview will be useful to those looking to employ optogenetics as a research tool.</p>
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			<media:title type="html">mariasmit</media:title>
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		<title>Using μMRI to Construct Atlases of Animal Development</title>
		<link>http://cshbenchmarks.wordpress.com/2011/03/01/using-%ce%bcmri-to-construct-atlases-of-animal-development/</link>
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		<pubDate>Tue, 01 Mar 2011 21:06:53 +0000</pubDate>
		<dc:creator>Bench Marks</dc:creator>
				<category><![CDATA[Developmental Biology]]></category>
		<category><![CDATA[Imaging/Microscopy]]></category>
		<category><![CDATA[Laboratory Organisms]]></category>

		<guid isPermaLink="false">http://cshbenchmarks.wordpress.com/?p=1765</guid>
		<description><![CDATA[The cover of the March 2011 issue of Cold Spring Harbor Protocols, out today, features several striking images of mouse and quail embryos.  The method used to produce the images, microscopic magnetic resonance imaging (μMRI), is a noninvasive imaging technique that permits the visualization of regions deep within embryos that are inaccessible using optical methods.  [...]<img alt="" border="0" src="http://stats.wordpress.com/b.gif?host=cshbenchmarks.wordpress.com&amp;blog=20090526&amp;post=1765&amp;subd=cshbenchmarks&amp;ref=&amp;feed=1" width="1" height="1" />]]></description>
			<content:encoded><![CDATA[<p><a href="http://cshprotocols.cshlp.org/TOCs/toc3_11.dtl">The cover of the March 2011 issue of <em>Cold Spring Harbor Protocols</em></a>, out today, features several striking images of mouse and quail embryos.  The method used to produce the images, microscopic magnetic resonance imaging (μMRI), is a noninvasive imaging technique that permits the visualization of regions deep within embryos that are inaccessible using optical methods.  During μMRI, the specimens remain in near-physiological conditions, remaining anatomically unperturbed.  The method is ideal, therefore, for generating developmental atlases of these organisms.</p>
<div id="attachment_1770" class="wp-caption aligncenter" style="width: 310px"><a href="http://cshbenchmarks.files.wordpress.com/2011/03/quail-embryos-for-umri.jpg"><img src="http://cshbenchmarks.files.wordpress.com/2011/03/quail-embryos-for-umri.jpg?w=300&#038;h=230" alt="" title="Quail Embryos for μMRI" width="300" height="230" class="size-medium wp-image-1770" /></a><p class="wp-caption-text">Quail embryos in a &quot;relaxed&quot; posture used to construct a μMRI-based developmental atlas. (©2011, CSHL Press)</p></div>
<p>In an <a href="http://cshprotocols.cshlp.org/cgi/content/abstract/2011/3/top100">accompanying article</a><em>, </em>the authors, Seth Ruffins and Russell Jacobs (<a href="http://bioimaging.caltech.edu/BIChome.html">Caltech Biological Imaging Center</a>), describe the preparation of specimens for μMRI and appropriate applications of μMRI for developmental biology, including the construction of atlases.  Using these methods, they have successfully generated digital anatomical atlases of both quail and mouse development (see the <a href="http://atlasserv.caltech.edu/">Caltech MRI Atlases</a>).  These atlases, and others constructed using μMRI, will be useful references for developmental biologists, providing identifiable anatomical landmarks and standards for comparison.</p>
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			<media:title type="html">mariasmit</media:title>
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