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	<title>neurodudes &#187; Neuroanatomy</title>
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	<link>http://neurodudes.com</link>
	<description>at the intersection of neuroscience and AI.</description>
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		<title>Crowdsourcing the Brain with the Whole Brain Catalog</title>
		<link>http://neurodudes.com/2009/10/24/crowdsourcing-the-brain-with-the-whole-brain-catalog/</link>
		<comments>http://neurodudes.com/2009/10/24/crowdsourcing-the-brain-with-the-whole-brain-catalog/#comments</comments>
		<pubDate>Sat, 24 Oct 2009 16:42:06 +0000</pubDate>
		<dc:creator>Stephen Larson</dc:creator>
				<category><![CDATA[At the scale of systems and functions]]></category>
		<category><![CDATA[Axons]]></category>
		<category><![CDATA[Dendrites]]></category>
		<category><![CDATA[Neural network models]]></category>
		<category><![CDATA[Neuroanatomy]]></category>
		<category><![CDATA[Neuronal arbors/neurites]]></category>
		<category><![CDATA[Systems biology]]></category>

		<guid isPermaLink="false">http://neurodudes.com/?p=814</guid>
		<description><![CDATA[A very cool article on a new open source, online system to crowd source the assemblage of data in neuroscience from the Voice of San Diego.  From the article: Traditionally, the study of the brain was organized somewhat like an archipelago. Neuroscientists would inhabit their own island or peninsula of the brain, and see little reason [...]]]></description>
			<content:encoded><![CDATA[<p><img class="alignnone" title="Whole Brain Catalog" src="http://bloximages.chicago2.vip.townnews.com/voiceofsandiego.org/content/tncms/assets/editorial/5/9e/5d1/59e5d108-ba6d-5a75-b966-91930c760555.image.jpg?_dc=1259852704" alt="" width="600" height="374" /></p>
<p>A very <a href="http://www.voiceofsandiego.org/articles/2009/10/24/science/869brain102209.txt">cool article</a> on a <a href="http://wholebraincatalog.org">new open source, online system</a> to <a href="http://en.wikipedia.org/wiki/Crowdsourcing">crowd source</a> the assemblage of data in neuroscience from the <a href="http://www.voiceofsandiego.org/">Voice of San Diego</a>.  From <a href="http://www.voiceofsandiego.org/articles/2009/10/24/science/869brain102209.txt">the article</a>:</p>
<blockquote><p>Traditionally, the study of the brain was organized somewhat like an archipelago. Neuroscientists would inhabit their own island or peninsula of the brain, and see little reason to venture elsewhere.</p>
<p>Molecular neuroscientists, who study how DNA and RNA function in the brain, didn&#8217;t share their work with cognitive specialists who study how psychological and cognitive functions are produced by the brain, for example.</p>
<p>But there has been an awakening to the idea that brains of humans and mammals should be studied like the complex, and interrelated systems that they are. Neuroscientists realized that they had to start collaborating across disciplines and sharing their data if they wanted to make advances in their own field.</p>
<p>[...]</p>
<p>Ellisman and his UCSD colleagues have devised a solution: crowdsource a brain. And this week they unveiled their years-long project &#8212; the <a style="color: #07467c; text-decoration: underline; font-weight: normal;" href="http://www.wholebraincatalog.org/" target="_blank">Whole Brain Catalog</a> &#8212; at the annual convention of the Society for Neuroscience, the largest gathering of brain experts in the world.</p></blockquote>
<p><span id="more-814"></span></p>
<p>You can also see an impressive  artists rendition of the <a href="http://www.youtube.com/watch?v=zXLeJFu57Wg">Whole Brain Catalog on YouTube</a>.</p>
<p>UPDATE 10/27: Looks like Voice of San Diego scooped the New York Times, who just posted on this topic <a href="http://www.google.com/url?sa=t&amp;source=web&amp;oi=news_result&amp;ct=res&amp;cd=1&amp;ved=0CAsQqQIwAA&amp;url=http%3A%2F%2Fbits.blogs.nytimes.com%2F2009%2F10%2F27%2Fa-virtual-voyage-through-the-brain-of-a-mouse%2F&amp;ei=3d7mSpKmKZHSsQPy8uTYCA&amp;usg=AFQjCNFCpKdkw-BJls7iPEtXgRMWqADpww&amp;sig2=rKxkuuGu2PJ-sTRsdtBySA">in today&#8217;s bits blog</a>.</p>
<p><em>Full disclosure: I am intimately involved with this project.</em></p>
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		<title>Frontiers in Neuroscience Journal</title>
		<link>http://neurodudes.com/2009/08/16/frontiers-in-neuroscience-journal/</link>
		<comments>http://neurodudes.com/2009/08/16/frontiers-in-neuroscience-journal/#comments</comments>
		<pubDate>Sun, 16 Aug 2009 21:02:16 +0000</pubDate>
		<dc:creator>Stephen Larson</dc:creator>
				<category><![CDATA[Brain-machine interfaces]]></category>
		<category><![CDATA[Cog/neuro science careers]]></category>
		<category><![CDATA[Computation within single neurons]]></category>
		<category><![CDATA[Computational neuroscience]]></category>
		<category><![CDATA[Conferences]]></category>
		<category><![CDATA[Consumer neurotechnology]]></category>
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		<category><![CDATA[Evolution]]></category>
		<category><![CDATA[Genetics and molecular]]></category>
		<category><![CDATA[Interdisciplinary concepts]]></category>
		<category><![CDATA[Internet and blogs]]></category>
		<category><![CDATA[Ion channels]]></category>
		<category><![CDATA[Jobs]]></category>
		<category><![CDATA[Medicine and other intervention/augmentation]]></category>
		<category><![CDATA[Memory and learning]]></category>
		<category><![CDATA[Methods and techniques]]></category>
		<category><![CDATA[Networks]]></category>
		<category><![CDATA[Neural development]]></category>
		<category><![CDATA[Neural network models]]></category>
		<category><![CDATA[Neural regeneration/neurogenesis]]></category>
		<category><![CDATA[Neuroanatomy]]></category>
		<category><![CDATA[Neuroengineering]]></category>
		<category><![CDATA[Neuronal arbors/neurites]]></category>
		<category><![CDATA[Neuropharmacology]]></category>
		<category><![CDATA[News, conferences, books, jobs, etc]]></category>
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		<guid isPermaLink="false">http://neurodudes.com/?p=767</guid>
		<description><![CDATA[The journal, Frontiers in Neuroscience, edited by Idan Segev, has made it Volume 3, issue 1.  Launching last year at the Society for Neuroscience conference, its probably the newest Neuroscience-related journal. I&#8217;m a fan of it because it is an open-access journal featuring a &#8220;tiered system&#8221; and more.  From their website: The Frontiers Journal Series [...]]]></description>
			<content:encoded><![CDATA[<p>The journal, <a href="http://www.frontiersin.org/neuroscience/">Frontiers in Neuroscience</a>, edited by Idan Segev, has made it Volume 3, issue 1.  Launching last year at the Society for Neuroscience conference, its probably the newest Neuroscience-related journal.</p>
<p>I&#8217;m a fan of it because it is an open-access journal featuring a &#8220;tiered system&#8221; and more.  <a href="http://www.frontiersin.org/aboutfrontiers/">From their website</a>:</p>
<blockquote><p>The Frontiers Journal Series is not just another journal. It is a new approach to scientific publishing. As service to scientists, it is driven by researchers for researchers but it also serves the interests of the general public. <strong>Frontiers </strong>disseminates research in a <a style="text-decoration: none;" href="http://www.frontiersin.org/publishingprocess/"><span style="color: #000000;">tiered system</span></a> that begins with original articles submitted to Specialty Journals. It <a style="text-decoration: none;" href="http://www.frontiersin.org/evaluationsystem/"><span style="color: #000000;">evaluates</span></a> research truly democratically and objectively based on the reading activity of the scientific communities and the public. And it drives the most outstanding and relevant research up to the next tier journals, <a style="font-size: 12px; list-style-type: none; list-style-position: initial; list-style-image: initial; text-decoration: none; padding: 0px;" href="http://www.frontiersin.org/"><span style="color: #000000;">the Field Journals</span></a><span style="color: #000000;">.</span></p></blockquote>
<p><span id="more-767"></span></p>
<p>I&#8217;m a big fan of the variety of specialty journals they have:</p>
<ul>
<li>Aging Neuroscience</li>
<li>Behavioral Neuroscience</li>
<li>Cellular Neuroscience</li>
<li>Computational Neuroscience</li>
<li>Enteric Neuroscience</li>
<li>Evolutionary Neuroscience</li>
<li>Human Neuroscience</li>
<li>Integrative Neuroscience</li>
<li>Molecular Neuroscience</li>
<li>Neural Circuits</li>
<li>Neuroanatomy</li>
<li>Neuroenergetics</li>
<li>Neuroengineering</li>
<li>Neurogenesis</li>
<li>Neurogenomics</li>
<li>Neuroinformatics</li>
<li>Neuromethods</li>
<li>Neuropharamacology</li>
<li>Neuroprosthetics</li>
<li>Neurorobotics</li>
<li>Synaptic Neuroscience</li>
<li>Systems Neuroscience</li>
</ul>
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		<title>Two color MARCM differentiates sister cells</title>
		<link>http://neurodudes.com/2009/07/18/two-color-marcm-differentiates-sister-cells/</link>
		<comments>http://neurodudes.com/2009/07/18/two-color-marcm-differentiates-sister-cells/#comments</comments>
		<pubDate>Sat, 18 Jul 2009 20:32:18 +0000</pubDate>
		<dc:creator>Neville Sanjana</dc:creator>
				<category><![CDATA[Genetics and molecular]]></category>
		<category><![CDATA[Methods and techniques]]></category>
		<category><![CDATA[Neural development]]></category>
		<category><![CDATA[Neuroanatomy]]></category>

		<guid isPermaLink="false">http://neurodudes.com/?p=728</guid>
		<description><![CDATA[Twin-spot MARCM to reveal the developmental origin and identity of neurons [Nature Neuro] We mentioned the innovative MARCM technique in a previous post. Here, Lee and colleagues extend MARCM (Mosaic Analysis with a Repressible Cell Marker, pronounced mark-em) to twin-spot MARCM, where both cells from a mitotic event are labeled with different colors fluorescent proteins. [...]]]></description>
			<content:encoded><![CDATA[<p><img class="alignnone size-full wp-image-729" title="Twin-spot MARCM" src="http://neurodudes.com/wp-content/uploads/2009/07/Picture-2.png" alt="Twin-spot MARCM" width="450" height="194" /><br />
<a href="http://www.nature.com/neuro/journal/v12/n7/full/nn.2345.html"> Twin-spot MARCM to reveal the developmental origin and identity of neurons</a> [Nature Neuro]</p>
<p>We mentioned the innovative MARCM technique <a href="http://neurodudes.com/2009/05/10/sunday-afternoon-reading-genetic-tools-primer/">in a previous post</a>. Here, Lee and colleagues extend MARCM (Mosaic Analysis with a Repressible Cell Marker, pronounced <em>mark-em</em>) to twin-spot MARCM, where both cells from a mitotic event are labeled with different colors fluorescent proteins. In regular MARCM, only one cell is labeled and the other daughter cell remained unlabeled. Like <a href="http://dx.doi.org/10.1016/S0166-2236(00)01791-4">the original MARCM</a>, this technique lets you distinguish between what would otherwise be identical pairs/clonal populations of cells during development and gain insight into the (lack of) stereotypy in development. Under the hood, twin-spot MARCM is a bit different: Instead of relying on GAL80 suppression of GAL4-driven transcription (regular MARCM), twin-spot MARCM uses RNAi directed against the protein-coding transcripts.</p>
<p>Since MARCM can be difficult to understand, here&#8217;s <a href="http://www.biol.sc.edu/~vogt/courses/neuro/neurolabs.html">an excellent, detailed yet easy-to-understand description</a> written for a bio lab class from <a href="http://www.biol.sc.edu/faculty/vogt.html">Richard Vogt at the University of South Carolina</a>:</p>
<blockquote>
<ol>
<li>A fly is constructed with the following genotype: (promotor)Gal4; UAS-GFP. In this fly, the promoter drives the expression of a transcription factor called Gal4, and Gal4 binds to and activates a regulatory site referred to as &#8220;UAS&#8221; (upstream activating sequence). Activation of the UAS site drives expression of GFP (green fluorescent protein) which fluoresces green when stimulated by blue light.</li>
<li>This fly also contains a gene encoding and expressing a protein called &#8220;Gal80&#8243;; Gal80 suppresses the action of Gal4. If Gal80 is expressed, no GFP is made and no green fluorescence can occur.</li>
<li>This fly also contains a complex of genes referred to as the FLP/FRT system; FLP is a transcription factor that activates the FRT site, which is situated adjacent to the Gal80 site. Further more, at least in our case, the FLP is driven by a &#8220;heat shock&#8221; promoter (hs). All this means is that when you raise the temperature of the animal to 37<sup>o</sup>C, this activates the hs promoter which activates the expression of FLP which activates the FRT site.
<p> &nbsp; &nbsp; &nbsp; &nbsp; <strong>Something I&#8217;ve not mentioned yet&#8230;</strong> there is also an FRT site adjacent to the UAS-GFP site. Something else I&#8217;ve not mentioned yet, the FRT-UAS-GFP site and the FRT-Gal80 site are on the same chromosome, but importantly on different chromatids.</p>
</li>
<li> So we make a bunch of fly embryos that have all this stuff in them. Procedurally this is really easy, since the genes have already been put in the flies, and all we have to do is take virgin females of one stain (FRT-Gal80) and mate them to males of another strain (FRT-UAS-GFP) and&#8230; POW&#8230; we have fly embryos that have all this stuff in them.</li>
<li>All the cells in the embryos we now have are capable of expressing GFP except for the one problem&#8230; all the cells are expressing Gal80 which is blocking the expression of GFP. We need to turn off Gal80 expression. We do this by activating the FLP/FRT system.</li>
<li> Normally, a cell has two copies of each chromosome called chromatids. In our case, the chromatids are different, one containing by FRT-Gal80 and the other containing FRT-UAS-GFP. This cell can not express GFP because Gal80 is present. During mitosis, the chromatids are duplicated and sort to produce two identical chromatid pairs, both pairs consisting of a FRT-Gal80 chromatid and a FRT-UAS-GFP chromatid. Like their mother, neither daughter cell would be able to express GFP, again because Gal80 is present.
<p> &nbsp; &nbsp; &nbsp; &nbsp; <strong>HOWEVER, AND HERE IS THE TRICK&#8230;</strong> if the FRT is activated during mitosis, it induces a recombination event (recombination normally only occurs during meiosis), creating one chromatid pair that contains only UAS-GFP and another chromatid pair that contains only Gal80. One of the resulting daughter cells now contains no Gal80, and suddenly is able to express GFP and fluoresce green light. And any additional cells produced by this daughter will also express GFP.</p>
</li>
</ol>
</blockquote>
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		<item>
		<title>The plan for H.M.&#8217;s brain</title>
		<link>http://neurodudes.com/2009/07/06/the-plan-for-h-m-s-brain/</link>
		<comments>http://neurodudes.com/2009/07/06/the-plan-for-h-m-s-brain/#comments</comments>
		<pubDate>Mon, 06 Jul 2009 14:11:12 +0000</pubDate>
		<dc:creator>Neville Sanjana</dc:creator>
				<category><![CDATA[Memory and learning]]></category>
		<category><![CDATA[Neuroanatomy]]></category>

		<guid isPermaLink="false">http://neurodudes.com/?p=716</guid>
		<description><![CDATA[Recently, the most famous (and most studied) person in neuroscience died. Science has a nice piece on the planning and post-morten examination of this most famous brain: [Suzanne] Corkin delivered Cryopaks to his nursing home in Windsor Locks, Connecticut. &#8220;They kept them in the freezer so that the moment he died they could wrap his [...]]]></description>
			<content:encoded><![CDATA[<p>Recently, <a href="http://en.wikipedia.org/wiki/HM_(patient)">the most famous (and most studied) person in neuroscience</a> died. <em>Science</em> has <a href="http://www.sciencemag.org/cgi/content/full/324/5935/1634">a nice piece on the planning and post-morten examination</a> of this most famous brain:</p>
<blockquote><p><a href="http://web.mit.edu/bnl/">[Suzanne] Corkin</a> delivered<sup> </sup>Cryopaks to his nursing home in Windsor Locks, Connecticut.<sup> </sup>&#8220;They kept them in the freezer so that the moment he died they<sup> </sup>could wrap his head to preserve the brain,&#8221; she says. When Molaison<sup> </sup>[ie. H.M.] died of respiratory failure at 5:05 p.m. on 8 December 2008,<sup> </sup>the plan sprang into action. A hearse took his body to Massachusetts<sup> </sup>General Hospital (MGH) in Charlestown, where researchers began<sup> </sup>collecting anatomical magnetic resonance imaging (MRI) scans<sup> </sup>of his brain at about 9 p.m.—and continued until 6 a.m.<sup> </sup>the next day, when Annese arrived on a red-eye flight from San<sup> </sup>Diego.</p></blockquote>
<p>Jacopo Annese, a neuroanatomist at UCSD, is planning on putting H.M.&#8217;s whole brain online <a href="http://thebrainobservatory.ucsd.edu/">on his website</a>. But before that happens, he has a rather huge task before him:</p>
<blockquote><p>Using<sup> </sup>a microtome, he will slice the brain into very thin sections.<sup> </sup>&#8220;Like prosciutto,&#8221; he says, but less than 1/20 the thickness<sup> </sup>and a lot more fragile. Annese aims to slice the brain whole<sup> </sup>instead of first cutting it into smaller chunks as is more routinely<sup> </sup>done. Small chunks are much easier to work with, but the resulting<sup> </sup>slices are hard to keep in register with one another. Whole-brain<sup> </sup>slices will keep more of the tissue intact and result in a more<sup> </sup>faithful reconstruction of the brain, he says.<sup> </sup> Annese estimates he will end up with about 2600 slices of Molaison&#8217;s<sup> </sup>brain. He and his colleagues will mount some of these, perhaps<sup> </sup>every 12th one to start, on extra-large glass slides—13<sup> </sup>by 18 centimeters—and treat them with a stain that colors<sup> </sup>cell bodies purple. A camera attached to a microscope will photograph<sup> </sup>each slice at 20<span style="font-family: arial,helvetica;">x</span> magnification, sufficient to distinguish different<sup> </sup>cell types. At that magnification, photographing a single slice<sup> </sup>will require a mosaic of about 40,000 individual images.</p></blockquote>
<p>And there is some stress that comes from dealing with such a one-of-a-kind specimen:</p>
<blockquote><p>But a lot could go wrong. The MRI scans reveal<sup> </sup>deterioration of the white matter, Annese says, which might<sup> </sup>make the slices especially delicate and prone to tearing. An<sup> </sup>even more nightmarish scenario is a cracked brain, he says.<sup> </sup>Sometimes, a brain will freeze unevenly and break apart—destroying<sup> </sup>it before it can be sliced. Annese is taking every precaution,<sup> </sup>but he&#8217;s not taking anything for granted. &#8220;Cutting will make<sup> </sup>or break the project,&#8221; he says. &#8220;But if the brain cracks, I<sup> </sup>go back to Italy.&#8221;</p></blockquote>
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