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		<id>http://istoriya.soippo.edu.ua/index.php?action=history&amp;feed=atom&amp;title=Gsk126_Sigma</id>
		<title>Gsk126 Sigma - Історія редагувань</title>
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		<updated>2026-04-10T15:17:08Z</updated>
		<subtitle>Історія редагувань цієї сторінки в вікі</subtitle>
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	<entry>
		<id>http://istoriya.soippo.edu.ua/index.php?title=Gsk126_Sigma&amp;diff=219274&amp;oldid=prev</id>
		<title>Star7dirt в 17:41, 22 серпня 2017</title>
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				<updated>2017-08-22T17:41:00Z</updated>
		
		<summary type="html">&lt;p&gt;&lt;/p&gt;
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				&lt;td colspan='2' style=&quot;background-color: white; color:black; text-align: center;&quot;&gt;← Попередня версія&lt;/td&gt;
				&lt;td colspan='2' style=&quot;background-color: white; color:black; text-align: center;&quot;&gt;Версія за 17:41, 22 серпня 2017&lt;/td&gt;
				&lt;/tr&gt;&lt;tr&gt;&lt;td colspan=&quot;2&quot; class=&quot;diff-lineno&quot;&gt;Рядок 1:&lt;/td&gt;
&lt;td colspan=&quot;2&quot; class=&quot;diff-lineno&quot;&gt;Рядок 1:&lt;/td&gt;&lt;/tr&gt;
&lt;tr&gt;&lt;td class='diff-marker'&gt;−&lt;/td&gt;&lt;td style=&quot;color:black; font-size: 88%; border-style: solid; border-width: 1px 1px 1px 4px; border-radius: 0.33em; border-color: #ffe49c; vertical-align: top; white-space: pre-wrap;&quot;&gt;&lt;div&gt;&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;Th secondary anti&lt;/del&gt;-&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;mouse IgG-AF488 (1:1000) in PS for 1 h&lt;/del&gt;, &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;plus &lt;/del&gt;the &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;nuclei have been stained by Hoechst 33258 (1:10000) for high-content automated microscopy. This method (referred &lt;/del&gt;to &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;as Pinda/perm HA) efficiently distinguishes involving &lt;/del&gt;the &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;endocytosed &lt;/del&gt;and &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;also &lt;/del&gt;the &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;non-internalized particles&lt;/del&gt;. &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;In manage samples&lt;/del&gt;, &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;the antibody staining was carried out exclusively either in PS &lt;/del&gt;(&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;perm Pinda/perm HA) or in BS (Pinda/HA&lt;/del&gt;). In &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;cells following &lt;/del&gt;the &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;perm Pinda/perm HA process, the endocytosed virus particles couldn't be distinguished &lt;/del&gt;in the &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;non-internalized particles&lt;/del&gt;. &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;In Pinda/HA cells, only the noninternalized particles had been detected. 3. Acidification (EA assay). The cells had been permeabilized with PS for 30 min at RT. The cells have been then incubated with mouse monoclonal A1 antibody &lt;/del&gt;in &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;PS (1:1000) for two h&lt;/del&gt;, &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;washed with PBS, and incubated with secondary anti-mouse IgG-AF488 (1:1000) in PS for 1 h together with either DRAQ5 (1:1000) or Hoechst 33258 (1:10000) in &lt;/del&gt;[http://www.ncbi.nlm.nih.gov/pubmed/&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;11967625 11967625&lt;/del&gt;] &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;PS&lt;/del&gt;. &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;four. Fusion (EF assay). IAV stocks have been diluted in PBS to 0.1 mg/ml &lt;/del&gt;and &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;labeled &lt;/del&gt;for &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;1 h at RT with R18 &lt;/del&gt;and &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;SP-DiOC18 (3) at final concentrations of 0&lt;/del&gt;.&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;four mM &lt;/del&gt;and &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;0&lt;/del&gt;.&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;two mM&lt;/del&gt;, &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;respectively&lt;/del&gt;. &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;The labeled virus particles had been filtered by way of a 0.22 mM-pore filter (Millipore) &lt;/del&gt;and &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;stored at 4uC &lt;/del&gt;in the &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;dark till use&lt;/del&gt;. &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;After internalization &lt;/del&gt;and &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;fixation, nuclei were stained with either DRAQ5 (1:1000) or Hoechst 33258 (1:10000) in BS&lt;/del&gt;. &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;5&lt;/del&gt;. &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;Uncoating (EU assay). The cell membrane &lt;/del&gt;was &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;stained with WGA-AF647 as described above. The cells have been permeabilized with PS for &lt;/del&gt;[&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;http://www&lt;/del&gt;.&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;ncbi.nlm.nih.gov/pubmed/1315463 1315463] 30 min at RT, &lt;/del&gt;and &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;incubated &lt;/del&gt;with &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;purified mouse monoclonal antibody HB64 in PS &lt;/del&gt;(&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;1:250&lt;/del&gt;) for &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;two h to stain &lt;/del&gt;the &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;viral M1. The cells have been washed with PBS&lt;/del&gt;, &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;followed &lt;/del&gt;by &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;incubation with secondary anti&lt;/del&gt;-&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;mouse IgG&lt;/del&gt;-&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;AF488 &lt;/del&gt;(&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;1:1000&lt;/del&gt;). &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;Nuclei had been stained with Hoechst 33258 (&lt;/del&gt;1&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;:10000)&lt;/del&gt;. &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;six&lt;/del&gt;. &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;Nuclear import &lt;/del&gt;(&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;EI assay&lt;/del&gt;). &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;The cells have &lt;/del&gt;been &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;permeabilized with PS &lt;/del&gt;for &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;30 &lt;/del&gt;min &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;at RT&lt;/del&gt;, and &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;incubated with mouse monoclonal antibody HB65 &lt;/del&gt;(&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;hybridoma supernatant&lt;/del&gt;) &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;in PS (1:10) for 2 h &lt;/del&gt;to &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;stain &lt;/del&gt;the &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;incoming viral NP&lt;/del&gt;. The &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;cells were washed with PBS, followed &lt;/del&gt;by &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;incubation with secondary anti-mouse IgG-AF488 (1&lt;/del&gt;:&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;1000)&lt;/del&gt;. &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;Nuclei were stained with either DRAQ5 (1:1000) or Hoechst 33258 (1:10000)&lt;/del&gt;. &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;7&lt;/del&gt;. &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;Infection. Newly synthesized NP was detected as described &lt;/del&gt;in &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;6&lt;/del&gt;.&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;High-Content Evaluation &lt;/del&gt;of &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;IAV Entry EventsImage AcquisitionFor high-resolution imaging&lt;/del&gt;, &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;specimen on coverslips &lt;/del&gt;from &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;24well plates had been mounted on a glass slide with Immu&lt;/del&gt;-&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;mount (Thermo Scientific) &lt;/del&gt;and &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;viewed on a Zeiss LSM 510 laser scanning confocal microscope&lt;/del&gt;. &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;Both 1006 and 636 objectives (1.four numerical aperture and 161 binning) were employed to obtain images. Automated image acquisition of 96-well Matrix plates &lt;/del&gt;was &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;performed having a 206objective &lt;/del&gt;(&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;0.75 numerical aperture and 161 binning) employing Molecular Devices ImageXpress Micro imaging technique. From each properly, 9 [https&lt;/del&gt;://&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;www&lt;/del&gt;.&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;medchemexpress&lt;/del&gt;.&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;com&lt;/del&gt;/&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;1-NM-PP1&lt;/del&gt;.&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;html 1-NM-PP1] photos (363&lt;/del&gt;) &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;were acquired for each and every channel&lt;/del&gt;.&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;Supporting InformationFigure S1 IAV binding within &lt;/del&gt;the &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;neuraminidase &lt;/del&gt;and &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;mocktreated cells. A549 cells &lt;/del&gt;were &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;treated &lt;/del&gt;with &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;0.25 units&lt;/del&gt;/&lt;del class=&quot;diffchange diffchange-inline&quot;&gt;ml neuraminidase at 37uC for four h&lt;/del&gt;, &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;followed by EB assay. Images &lt;/del&gt;have been &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;acquired &lt;/del&gt;having a &lt;del class=&quot;diffchange diffchange-inline&quot;&gt;confocal microscope&lt;/del&gt;.&lt;/div&gt;&lt;/td&gt;&lt;td class='diff-marker'&gt;+&lt;/td&gt;&lt;td style=&quot;color:black; font-size: 88%; border-style: solid; border-width: 1px 1px 1px 4px; border-radius: 0.33em; border-color: #a3d3ff; vertical-align: top; white-space: pre-wrap;&quot;&gt;&lt;div&gt;&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;Cterial cell wall is involved in PG cross&lt;/ins&gt;-&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;linking&lt;/ins&gt;, the &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;lack of or incorrect substrateincorporation in &lt;/ins&gt;to the &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;PG macromolecule can result in improperly constructed PG &lt;/ins&gt;and &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;in &lt;/ins&gt;the &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;end to cell death by means of lysis as a consequence of inability with the bacterium to preserve osmotic pressure [14,15]&lt;/ins&gt;. &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;Here we report the first characterization of a Mur ligase from the genus Verrucomicrobium&lt;/ins&gt;, &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;namely MurE from V. spinosum &lt;/ins&gt;(&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;MurEVs&lt;/ins&gt;). In &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;vivo analysis demonstrates that &lt;/ins&gt;the &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;enzyme is in a position to functionally complement an Escherichia coli strain that harbors a mutation &lt;/ins&gt;in the &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;murE gene&lt;/ins&gt;. &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;Employing &lt;/ins&gt;in &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;vitro analyses&lt;/ins&gt;, [http://www.ncbi.nlm.nih.gov/pubmed/&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;10457188 10457188&lt;/ins&gt;] &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;we show that MurEVs is a meso-A2pm-adding enzyme&lt;/ins&gt;. &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;Additionally, we present a structural analysis from the enzyme utilizing protein sequence alignment &lt;/ins&gt;and &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;homology modeling, which shows that key amino acids &lt;/ins&gt;for &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;substrate binding &lt;/ins&gt;and&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;/or catalysis are conserved in MurEVs&lt;/ins&gt;. &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;With each other, these experiments contribute to the additional understanding in the kinetic, physical &lt;/ins&gt;and &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;structural properties in the Mur ligase involved in the synthesis of PG in the organism V. spinosum&lt;/ins&gt;. &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;Lastly&lt;/ins&gt;, &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;V&lt;/ins&gt;. &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;spinosum PG was purified &lt;/ins&gt;and &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;analyzed; its composition &lt;/ins&gt;in &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;which A2pm is one of &lt;/ins&gt;the &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;principal constituents is equivalent to that of most Gram-negative bacteria&lt;/ins&gt;.&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;Materials &lt;/ins&gt;and &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;Techniques V&lt;/ins&gt;. &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;spinosum growth conditionsV&lt;/ins&gt;. &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;spinosum DSM 4136T &lt;/ins&gt;was &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;cultured in R2A medium at 26uC &lt;/ins&gt;[&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;10]&lt;/ins&gt;.&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;PCR amplification &lt;/ins&gt;and &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;cloning &lt;/ins&gt;with &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;the V. spinosum murE open reading frame &lt;/ins&gt;(&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;ORF&lt;/ins&gt;) for &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;protein expression and purificationThe open reading frame annotated by &lt;/ins&gt;the &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;locus tag (VspiD_010100019130) UDP-N-acetylmuramoyl-L-alanyl-D-glutamate:meso-2&lt;/ins&gt;,&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;6-diaminopimelate ligase was amplified &lt;/ins&gt;by &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;PCR. The following forward and reverse primers were applied: murEVs&lt;/ins&gt;-&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;forward 59&lt;/ins&gt;-&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;CACCATGACCATTTTGCGCGATCTTATCGAGGGT-39 and murEVs-reverse 59-GTCGACTCACTGACGGTCATCCCTCCTTTGGCGTGC-39 &lt;/ins&gt;(&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;the underlined sequence represents the restriction enzyme web page utilized to facilitate sub-cloning of your ORF whilst the bold and italicized sequences represent initiation and termination codons&lt;/ins&gt;). &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;The PCR reaction contained 12 pmol of forward and reverse primers, &lt;/ins&gt;1 &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;mM MgSO4, 0&lt;/ins&gt;.&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;five mM of each on the four deoxynucleotide triphosphates, 0&lt;/ins&gt;.&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;5 ng ofMurE from Verrucomicrobium spinosum DSM 4136Tgenomic DNA and 1 unit of Platinum Pfx DNA polymerase &lt;/ins&gt;(&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;Invitrogen Corporation, Carlsbad, CA, USA&lt;/ins&gt;). &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;PCR conditions had &lt;/ins&gt;been&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;: 1 cycle at 94uC &lt;/ins&gt;for &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;2 &lt;/ins&gt;min, &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;followed by 30 cycles of 94uC for 15 s, 60uC for 30 s &lt;/ins&gt;and &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;72uC for two min. The murE PCR fragment was ligated into the plasmid pET100D/topo &lt;/ins&gt;(&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;Invitrogen Corporation, Carlsbad, CA, USA&lt;/ins&gt;) to &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;make &lt;/ins&gt;the &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;plasmid pET100D::murEVs&lt;/ins&gt;. The &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;recombinant protein encoded &lt;/ins&gt;by &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;this plasmid carries a MRGSHHHHHHGMASMTGGQQMGRDLYDDDDKDHPFT sequence [https&lt;/ins&gt;:&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;//www&lt;/ins&gt;.&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;medchemexpress&lt;/ins&gt;.&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;com/Doxorubicin-hydrochloride&lt;/ins&gt;.&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;html Adriamycin site] containing a hexa-histidine tag derived &lt;/ins&gt;in &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;the pET100D plasmids in the amino terminus&lt;/ins&gt;. &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;To confirm the fidelity &lt;/ins&gt;of &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;the&amp;#160; PCR reaction&lt;/ins&gt;, &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;the murE ORF was sequenced &lt;/ins&gt;from &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;pET100D using the T7 promoter primer, 59TAATACGACTCACTATAGGG&lt;/ins&gt;-&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;39 &lt;/ins&gt;and &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;also the T7 reverse primer, 59-TAGTTATTGCTCAGCGGTGG-39&lt;/ins&gt;. &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;The cloned murE ORF &lt;/ins&gt;was &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;one hundred&amp;#160; identical for the sequences deposited in the Integrated Microbial Genomes public database &lt;/ins&gt;(&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;http&lt;/ins&gt;://&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;img&lt;/ins&gt;.&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;jgi&lt;/ins&gt;.&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;doe.gov&lt;/ins&gt;/&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;cgibin/w/main&lt;/ins&gt;.&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;cgi&lt;/ins&gt;).the &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;labeled substrate; in that case, radioactive substrate &lt;/ins&gt;and &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;product &lt;/ins&gt;were &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;separated by thin-layer chromatography on silica gel plates LK6D (Whatman) working &lt;/ins&gt;with &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;1-propanol&lt;/ins&gt;/&lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;ammonium hydroxide/water (six:3:1; v/v) because the mobile phase&lt;/ins&gt;, &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;and the radioactive spots &lt;/ins&gt;have been &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;positioned and quantified &lt;/ins&gt;having a &lt;ins class=&quot;diffchange diffchange-inline&quot;&gt;radioactivity scanner (Rita Star, Raytest Isotopenmebgerate GmbH)&lt;/ins&gt;.&lt;/div&gt;&lt;/td&gt;&lt;/tr&gt;
&lt;/table&gt;</summary>
		<author><name>Star7dirt</name></author>	</entry>

	<entry>
		<id>http://istoriya.soippo.edu.ua/index.php?title=Gsk126_Sigma&amp;diff=219147&amp;oldid=prev</id>
		<title>Grass7man: Створена сторінка: Th secondary anti-mouse IgG-AF488 (1:1000) in PS for 1 h, plus the nuclei have been stained by Hoechst 33258 (1:10000) for high-content automated microscopy. Th...</title>
		<link rel="alternate" type="text/html" href="http://istoriya.soippo.edu.ua/index.php?title=Gsk126_Sigma&amp;diff=219147&amp;oldid=prev"/>
				<updated>2017-08-22T12:27:00Z</updated>
		
		<summary type="html">&lt;p&gt;Створена сторінка: Th secondary anti-mouse IgG-AF488 (1:1000) in PS for 1 h, plus the nuclei have been stained by Hoechst 33258 (1:10000) for high-content automated microscopy. Th...&lt;/p&gt;
&lt;p&gt;&lt;b&gt;Нова сторінка&lt;/b&gt;&lt;/p&gt;&lt;div&gt;Th secondary anti-mouse IgG-AF488 (1:1000) in PS for 1 h, plus the nuclei have been stained by Hoechst 33258 (1:10000) for high-content automated microscopy. This method (referred to as Pinda/perm HA) efficiently distinguishes involving the endocytosed and also the non-internalized particles. In manage samples, the antibody staining was carried out exclusively either in PS (perm Pinda/perm HA) or in BS (Pinda/HA). In cells following the perm Pinda/perm HA process, the endocytosed virus particles couldn't be distinguished in the non-internalized particles. In Pinda/HA cells, only the noninternalized particles had been detected. 3. Acidification (EA assay). The cells had been permeabilized with PS for 30 min at RT. The cells have been then incubated with mouse monoclonal A1 antibody in PS (1:1000) for two h, washed with PBS, and incubated with secondary anti-mouse IgG-AF488 (1:1000) in PS for 1 h together with either DRAQ5 (1:1000) or Hoechst 33258 (1:10000) in [http://www.ncbi.nlm.nih.gov/pubmed/11967625 11967625] PS. four. Fusion (EF assay). IAV stocks have been diluted in PBS to 0.1 mg/ml and labeled for 1 h at RT with R18 and SP-DiOC18 (3) at final concentrations of 0.four mM and 0.two mM, respectively. The labeled virus particles had been filtered by way of a 0.22 mM-pore filter (Millipore) and stored at 4uC in the dark till use. After internalization and fixation, nuclei were stained with either DRAQ5 (1:1000) or Hoechst 33258 (1:10000) in BS. 5. Uncoating (EU assay). The cell membrane was stained with WGA-AF647 as described above. The cells have been permeabilized with PS for [http://www.ncbi.nlm.nih.gov/pubmed/1315463 1315463] 30 min at RT, and incubated with purified mouse monoclonal antibody HB64 in PS (1:250) for two h to stain the viral M1. The cells have been washed with PBS, followed by incubation with secondary anti-mouse IgG-AF488 (1:1000). Nuclei had been stained with Hoechst 33258 (1:10000). six. Nuclear import (EI assay). The cells have been permeabilized with PS for 30 min at RT, and incubated with mouse monoclonal antibody HB65 (hybridoma supernatant) in PS (1:10) for 2 h to stain the incoming viral NP. The cells were washed with PBS, followed by incubation with secondary anti-mouse IgG-AF488 (1:1000). Nuclei were stained with either DRAQ5 (1:1000) or Hoechst 33258 (1:10000). 7. Infection. Newly synthesized NP was detected as described in 6.High-Content Evaluation of IAV Entry EventsImage AcquisitionFor high-resolution imaging, specimen on coverslips from 24well plates had been mounted on a glass slide with Immu-mount (Thermo Scientific) and viewed on a Zeiss LSM 510 laser scanning confocal microscope. Both 1006 and 636 objectives (1.four numerical aperture and 161 binning) were employed to obtain images. Automated image acquisition of 96-well Matrix plates was performed having a 206objective (0.75 numerical aperture and 161 binning) employing Molecular Devices ImageXpress Micro imaging technique. From each properly, 9 [https://www.medchemexpress.com/1-NM-PP1.html 1-NM-PP1] photos (363) were acquired for each and every channel.Supporting InformationFigure S1 IAV binding within the neuraminidase and mocktreated cells. A549 cells were treated with 0.25 units/ml neuraminidase at 37uC for four h, followed by EB assay. Images have been acquired having a confocal microscope.&lt;/div&gt;</summary>
		<author><name>Grass7man</name></author>	</entry>

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