Help:Tutorial:Step 6

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==== 1. Stack the mCry/mPer DataNodes ====
==== 1. Stack the mCry/mPer DataNodes ====
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To illustrate that the mCry/mPer genes are activated by the E-box element, we can stack them below the 'Gene' label. Place the mPer/mCry DataNodes below the 'Gene' label and stack them in two vertical pairs, using the [[Image:stackverticalcenter.gif]] ''stack vertically'' button. Group each stacked pair.
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To illustrate that the mCry/mPer genes are activated by the E-box element, we can stack them below the 'Gene' label. Place the mPer/mCry DataNodes below the 'Gene' label and stack them in two vertical pairs, using the {{TutorialImage|stackverticalcenter.gif}} ''stack vertically'' button. Group each stacked pair.
==== 2. Copy the gene-products ====
==== 2. Copy the gene-products ====
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As long as Per1 or Per2 is not dimerized with Cry1 or Cry2, it will be degraded. We can indicate degradation by using the ''degradation'' shape:
As long as Per1 or Per2 is not dimerized with Cry1 or Cry2, it will be degraded. We can indicate degradation by using the ''degradation'' shape:
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You will notice that this shape is not on the toolbar, so to insert it, we have to insert another shape (e.g. a rectangle) and change it's ''Shape Type'' property. Insert a rectangle, select it and change the ''Shape Type'' property in the [[Help:Tutorial#Used terms and abbreviations|properties table]] to ''mim-degradation'':
You will notice that this shape is not on the toolbar, so to insert it, we have to insert another shape (e.g. a rectangle) and change it's ''Shape Type'' property. Insert a rectangle, select it and change the ''Shape Type'' property in the [[Help:Tutorial#Used terms and abbreviations|properties table]] to ''mim-degradation'':
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Revision as of 17:10, 13 May 2010


Next step | Index

Target genes are activated by the E-box element

After the Clock/Bmal1 dimer binds to the E-box element, transcription of several target genes are activated. This simplified version of the Circadian clock pathway, will restrict to the mPer/mCry genes, which will act as a negative feedback loop. As long as Per1 or Per2 exist as monomers, they will be phosphorylated by casein kinase 1 delta or epsilon, followed by degradation. In the pathway drawing we simplify it a bit by leaving out the phosphorylation event, resulting in the following representation:

transcription_degradation.png
Drawing the transcription of mPer/mCry
and degradation of mPer

1. Stack the mCry/mPer DataNodes

To illustrate that the mCry/mPer genes are activated by the E-box element, we can stack them below the 'Gene' label. Place the mPer/mCry DataNodes below the 'Gene' label and stack them in two vertical pairs, using the stackverticalcenter.gif stack vertically button. Group each stacked pair.

2. Copy the gene-products

The genes will be translated into proteins, to show this on the pathway, copy the stacked genes and move them to the right of the stacked DataNodes.

3. Draw a line from the genes to the gene-products

To illustrate that the genes are translated into proteins, we draw a dashed arrow from each pair of genes to the copied pair. Connect the start and end points to the groups.

5. Create a degradation shape

As long as Per1 or Per2 is not dimerized with Cry1 or Cry2, it will be degraded. We can indicate degradation by using the degradation shape:

degradation.png

You will notice that this shape is not on the toolbar, so to insert it, we have to insert another shape (e.g. a rectangle) and change it's Shape Type property. Insert a rectangle, select it and change the Shape Type property in the properties table to mim-degradation:

shapetype.png

When you selected mim-degradation as property, you will see the rectangle change into a degradation shape.

6. Draw an arrow from the mPer DataNodes to the degradation shape

To show that the mPer proteins are degraded, draw an dashed arrow from the two mPer DataNodes to the degradation shape. Connect the start of this line to group 2.1 to specify that only the mPer proteins are degraded.

Next step | Index

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