<div dir="ltr"><div><div>Hi Bassem,<br></div> The concentration suiting for negative-stain observation ranges from 50nM to 100nM.<br></div>--Zheng<br></div><div class="gmail_extra"><br clear="all"><div><div class="gmail_signature"><div dir="ltr">Zheng Liu Ph.D.<br>Postdoc, The Frank Lab<br>Department of Biochemistry & Molecular Biophysics<br>Columbia University<br><a href="http://franklab.cpmc.columbia.edu/franklab/" target="_blank">http://franklab.cpmc.columbia.edu/franklab/</a><br></div></div></div>
<br><div class="gmail_quote">On Wed, Jul 8, 2015 at 11:52 AM, Shebl, Bassem M. (MU-Student) <span dir="ltr"><<a href="mailto:bmgmw7@mail.missouri.edu" target="_blank">bmgmw7@mail.missouri.edu</a>></span> wrote:<br><blockquote class="gmail_quote" style="margin:0 0 0 .8ex;border-left:1px #ccc solid;padding-left:1ex">
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Dear all,
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<div>I am a new student to the field of electron microscopy. As a part of a project to an electron microscopy course I am taking, we are trying to look at negatively stained ribosomes. Does anyone have experience regarding this? Buffers used, concentrations,
stain used? I did search the literature few times to look for recent publications on the topic but didn’t come across anything useful. I started with 2% Uranyl Acetate in “20 mM HEPESKOH (pH 7.5), 6 mM MgCl<span style="vertical-align:-1pt">2</span>, 150
mM NH<span style="vertical-align:-1pt">4</span>Cl, 6 mM b-mercaptoethanol, 2 mM spermidine, and 0.1 mM spermine” with a concentration of 15 nM. </div><span class="HOEnZb"><font color="#888888">
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<div>Bassem Shebl<br>
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