Berglund:Protocols: Difference between revisions

Revision as of 09:43, 7 March 2014

http://openwetware.org/wiki/Berglund_Lab

Gels horizontal gels Agarose Denaturing Agarose vertical gels SDS-PAGE Denaturing Acrylamide Native Acrylamide Acrylamide-Agarose Native gels for in vivo splicing	Nucleic Acid DNA PCR: Commonly Used Primers Plasmids PCR: Various Methods RNA Transcription: Various Methods calculating RNA molecular weight RNA column purification making rNTP Labelling and Cleanup Kinasing Phenol/Ethanol Extraction Blots Northern Blot	Structure Footprinting UV crosslinking SHAPE (finished protocol) Analytical computer programs
Protein preparing your proteins Protein Buffers Protein Purification: Various Methods Protein Concentration Assay: Various Methods staining gels Coomassie Blue Staining Silverstaining using your protein GST pulldown example Binding Gels: Various Methods Western Blot	Cloning and Bacteria Cells Available Making Competent Cells: Various Methods Chemical Transformation Cloning: Various Methods Plasmids NEB sheets for enzyme cutting	General Recipes Buffers Worm Fix 2xDenaturing Dye Spec and Qubit calculators Calculating solutions Calculating protein concentrations
Antibody Work List of Antibodies Available Antibody Storage Antibody Purification Antibody Making/Ordering	Splicing In Vivo Proper cell culture technique In Vivo Cells Available General Cell Culture Methods Harvesting RNA Post-Harvesting RNA Freezing cells In Vitro Background Complex Formation Splicing	Equipment Using the TEM Equipment available

@@ Line 7: / Line 7: @@
 <!--------------------------------Gels ---------------------------------->
 <!------------------------------------------------------------------------------->
-== Gels ==
+<big><big>Gels</big></big>
-[[Berglund:Agarose|<h3><font color=#000000>Agarose</font></h3>]]
+----
-[[Berglund:SDS-PAGE|<h3><font color=#000000>SDS-PAGE</font></h3>]]
+horizontal gels
-[[Berglund:Acrylamide|<h3><font color=#000000>Acrylamide</font></h3>]]
+:[[Berglund:Agarose|<h3><font color=#000000>Agarose</font></h3>]]
-[[Berglund:Native Acrylamide|<h3><font color=#000000>Native Acrylamide</font></h3>]]
+:[[Berglund:Denaturing Agarose|<h3><font color=#000000>Denaturing Agarose</font></h3>]]
-[[Berglund:Acrylamide-Agarose|<h3><font color=#000000>Acrylamide-Agarose</font></h3>]]
+vertical gels
+:[[Berglund:SDS-PAGE|<h3><font color=#000000>SDS-PAGE</font></h3>]]
+:[[Berglund:Acrylamide|<h3><font color=#000000>Denaturing Acrylamide</font></h3>]]
+:[[Berglund:Native Acrylamide|<h3><font color=#000000>Native Acrylamide</font></h3>]]
+:[[Berglund:Acrylamide-Agarose|<h3><font color=#000000>Acrylamide-Agarose</font></h3>]]
+:[[Berglund:Native gels for in vivo splicing|<h3><font color=#000000>Native gels for in vivo splicing</font></h3>]]
@@ Line 22: / Line 27: @@
 <!------------------------------------------------------------------------------->
-== Nucleic Acid==
+<big><big>Nucleic Acid</big></big>
-[[Berglund:PCR: Commonly Used Primers|<h3><font color=#000000>PCR: Commonly Used Primers</font></h3>]]
+----
-[[Berglund:PCR: Various Methods|<h3><font color=#000000>PCR: Various Methods</font></h3>]]
+DNA
-[[Berglund:Transcription: Various Methods|<h3><font color=#000000>Transcription: Various Methods</font></h3>]]
+:[[Berglund:PCR: Commonly Used Primers|<h3><font color=#000000>PCR: Commonly Used Primers</font></h3>]]
-[[Berglund:Kinasing|<h3><font color=#000000>Kinasing</font></h3>]]
+:[[Berglund:Plasmids|<h3><font color=#000000>Plasmids</font></h3>]]
-[[Berglund:Phenol/Ethanol Extraction|<h3><font color=#000000>Phenol/Ethanol Extraction</font></h3>]]
+:[[Berglund:PCR: Various Methods|<h3><font color=#000000>PCR: Various Methods</font></h3>]]
-[[Berglund:RNA column purification|<h3><font color=#000000>RNA column purification</font></h3>]]
+RNA
-[[Berglund: making rNTP|<h3><font color=#000000>making rNTP</font></h3>]]
+:[[Berglund:Transcription: Various Methods|<h3><font color=#000000>Transcription: Various Methods</font></h3>]]
+:[[Berglund: calculating RNA molecular weight|<h3><font color=#000000>calculating RNA molecular weight</font></h3>]]
+:[[Berglund:RNA column purification|<h3><font color=#000000>RNA column purification</font></h3>]]
+:[[Berglund: making rNTP|<h3><font color=#000000>making rNTP</font></h3>]]
+Labelling and Cleanup
+:[[Berglund:Kinasing|<h3><font color=#000000>Kinasing</font></h3>]]
+:[[Berglund:Phenol/Ethanol Extraction|<h3><font color=#000000>Phenol/Ethanol Extraction</font></h3>]]
+Blots
+:[[Berglund: Northern Blot|<h3><font color=#000000>Northern Blot</font></h3>]]
 </div>
 |width="33%" style="border: 1px solid #ff3333; color: #000; background-color: #FFFFFF"|
@@ Line 39: / Line 52: @@
 <!------------------------------------------------------------------------------->
-== Structure==
+<big><big>Structure</big></big>
+----
 [[Berglund:Footprinting|<h3><font color=#000000>Footprinting</font></h3>]]
 [[Berglund:UV crosslinking|<h3><font color=#000000>UV crosslinking</font></h3>]]
-[[Berglund:SHAPE|<h3><font color=#000000>SHAPE</font></h3>]]
+[[Berglund:SHAPE2|<h3><font color=#000000>SHAPE (finished protocol)</font></h3>]]
-[[Berglund:Crystallography|<h3><font color=#000000>Crystallography</font></h3>]]
 [[Berglund:Analytical computer programs|<h3><font color=#000000>Analytical computer programs</font></h3>]]
@@ Line 55: / Line 68: @@
 <!------------------------------------------------------------------------------->
-==Protein==
+<big><big>Protein</big></big>
-[[Berglund:Protein Buffers|<h3><font color=#000000>Protein Buffers</font></h3>]]
+----
-[[Berglund:Protein Purification: Various Methods|<h3><font color=#000000>Protein Purification: Various Methods</font></h3>]]
+preparing your proteins
-[[Berglund:Binding Gels: Various Methods|<h3><font color=#000000>Binding Gels: Various Methods</font></h3>]]
+:[[Berglund:Protein Buffers|<h3><font color=#000000>Protein Buffers</font></h3>]]
-[[Berglund:Protein Concentration Assay: Various Methods|<h3><font color=#000000>Protein Concentration Assay: Various Methods</font></h3>]]
+:[[Berglund:Protein Purification: Various Methods|<h3><font color=#000000>Protein Purification: Various Methods</font></h3>]]
-[[Berglund:Western Blot|<h3><font color=#000000>Western Blot</font></h3>]]
+:[[Berglund:Protein Concentration Assay: Various Methods|<h3><font color=#000000>Protein Concentration Assay: Various Methods</font></h3>]]
-[[Berglund:Coomassie Blue Staining|<h3><font color=#000000>Coomassie Blue Staining</font></h3>]]
+staining gels
-[[Berglund:Silverstaining|<h3><font color=#000000>Silverstaining</font></h3>]]
+:[[Berglund:Coomassie Blue Staining|<h3><font color=#000000>Coomassie Blue Staining</font></h3>]]
+:[[Berglund:Silverstaining|<h3><font color=#000000>Silverstaining</font></h3>]]
+using your protein
+:[[Berglund:GST pulldown example|<h3><font color=#000000>GST pulldown example</font></h3>]]
+:[[Berglund:Binding Gels: Various Methods|<h3><font color=#000000>Binding Gels: Various Methods</font></h3>]]
+:[[Berglund:Western Blot|<h3><font color=#000000>Western Blot</font></h3>]]
 </div>
@@ Line 72: / Line 89: @@
 <!------------------------------------------------------------------------------->
-==Cloning and Bacteria==
+<big><big>Cloning and Bacteria</big></big>
+----
 [[Berglund:Cells Available|<h3><font color=#000000>Cells Available</font></h3>]]
 [[Berglund:Making Competent Cells: Various Methods|<h3><font color=#000000>Making Competent Cells: Various Methods</font></h3>]]
 [[Berglund:Chemical Transformation|<h3><font color=#000000>Chemical Transformation</font></h3>]]
-[[Berglund:Electroporation|<h3><font color=#000000>Electroporation</font></h3>]]
 [[Berglund:Cloning: Various Methods|<h3><font color=#000000>Cloning: Various Methods</font></h3>]]
+[[Berglund:Plasmids|<h3><font color=#000000>Plasmids</font></h3>]]
+[[Berglund:NEB sheets for enzyme cutting|<h3><font color=#000000>NEB sheets for enzyme cutting</font></h3>]]
 </div>
@@ Line 84: / Line 103: @@
 <div style="clear: right; text-align: left; float: left; padding: .1em 1.5em .9em">
 <!------------------------------------------------------------------------------->
-<!--------------------------------General---------------------------------->
+<!--------------------------------General Recipes---------------------------------->
 <!------------------------------------------------------------------------------->
-==General==
+<big><big>General Recipes</big></big>
+----
 [[Berglund:Buffers|<h3><font color=#000000>Buffers</font></h3>]]
-[[Berglund:Machines Available for Use|<h3><font color=#000000>Machines Available for Use</font></h3>]]
-[[Berglund:Formerly Used Protocols|<h3><font color=#000000>Formerly Used Protocols</font></h3>]]
 [[Berglund:Worm Fix|<h3><font color=#000000>Worm Fix</font></h3>]]
+[[Berglund:2xDenaturing Dye|<h3><font color=#000000>2xDenaturing Dye</font></h3>]]
+[[Berglund:Spec and Qubit calculators|<h3><font color=#000000>Spec and Qubit calculators</font></h3>]]
+[[Berglund:Calculating solutions|<h3><font color=#000000>Calculating solutions</font></h3>]]
+[[Berglund:Calculating protein concentrations|<h3><font color=#000000>Calculating protein concentrations</font></h3>]]
 </div>
 |-
@@ Line 101: / Line 123: @@
 <!------------------------------------------------------------------------------->
-==Antibody Work==
+<big><big>Antibody Work</big></big>
+----
 [[Berglund:List of Antibodies Available|<h3><font color=#000000>List of Antibodies Available</font></h3>]]
 [[Berglund:Antibody Storage|<h3><font color=#000000>Antibody Storage</font></h3>]]
@@ Line 114: / Line 137: @@
 <!------------------------------------------------------------------------------->
-==Splicing==
+<big><big>Splicing</big></big>
+----
 '''In Vivo'''<br>
-[[Berglund:Cells Available|<h3><font color=#000000>Cells Available</font></h3>]]
+:[[Berglund:Cell culture guide|<h3><font color=##CA0000>Proper cell culture technique</font></h3>]]
-[[Berglund:General Cell Culture Methods|<h3><font color=#000000>General Cell Culture Methods</font></h3>]]
+:[[Berglund:In Vivo Cells Available|<h3><font color=#000000>In Vivo Cells Available</font></h3>]]
-[[Berglund:Solutions|<h3><font color=#000000>Solutions</font></h3>]]
+:[[Berglund:General Cell Culture Methods|<h3><font color=#000000>General Cell Culture Methods</font></h3>]]
-[[Berglund:Methods of Analysis|<h3><font color=#000000>Methods of Analysis</font></h3>]]
+:[[Berglund:Harvesting RNA|<h3><font color=#000000>Harvesting RNA</font></h3>]]
+:[[Berglund:Post-Harvesting RNA|<h3><font color=#000000>Post-Harvesting RNA</font></h3>]]
+:[[Berglund:Freezing cells|<h3><font color=#000000>Freezing cells</font></h3>]]
 '''In Vitro'''<br>
-[[Berglund:Background|<h3><font color=#000000>Background</font></h3>]]
+:[[Berglund:Background|<h3><font color=#000000>Background</font></h3>]]
-[[Berglund:Complex Formation|<h3><font color=#000000>Complex Formation</font></h3>]]
+:[[Berglund:Complex Formation|<h3><font color=#000000>Complex Formation</font></h3>]]
-[[Berglund:Splicing|<h3><font color=#000000>Splicing</font></h3>]]
+:[[Berglund:Splicing|<h3><font color=#000000>Splicing</font></h3>]]
 </div>
@@ Line 133: / Line 159: @@
 <!------------------------------------------------------------------------------->
-==Nanoparticle Work==
+<big><big>Equipment</big></big>
+----
+[[Berglund:Using the TEM|<h3><font color=#000000>Using the TEM</font></h3>]]
+[[Berglund:Equipment available|<h3><font color=#000000>Equipment available</font></h3>]]
 </div>

Berglund:Protocols: Difference between revisions

Revision as of 09:43, 7 March 2014

Agarose

Denaturing Agarose

SDS-PAGE

Denaturing Acrylamide

Native Acrylamide

Acrylamide-Agarose

Native gels for in vivo splicing

PCR: Commonly Used Primers

Plasmids

PCR: Various Methods

Transcription: Various Methods

calculating RNA molecular weight

RNA column purification

making rNTP

Kinasing

Phenol/Ethanol Extraction

Northern Blot

Footprinting

UV crosslinking

SHAPE (finished protocol)

Analytical computer programs

Protein Buffers

Protein Purification: Various Methods

Protein Concentration Assay: Various Methods

Coomassie Blue Staining

Silverstaining

GST pulldown example

Binding Gels: Various Methods

Western Blot

Cells Available

Making Competent Cells: Various Methods

Chemical Transformation

Cloning: Various Methods

Plasmids

NEB sheets for enzyme cutting

Buffers

Worm Fix

2xDenaturing Dye

Spec and Qubit calculators

Calculating solutions

Calculating protein concentrations

List of Antibodies Available

Antibody Storage

Antibody Purification

Antibody Making/Ordering

Proper cell culture technique

In Vivo Cells Available

General Cell Culture Methods

Harvesting RNA

Post-Harvesting RNA

Freezing cells

Background

Complex Formation

Splicing

Using the TEM

Equipment available

Navigation menu

Search