Lidstrom:Sequencing with GeneWiz: Difference between revisions

Revision as of 16:29, 10 June 2014

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Price per rxn: $6 JM 10/2012

This is the standard UW price, but volume discounts are possible if our lab starts using more.

SUBMIT TO UW By REQUEST Box A

In summer of 2013 we got a GeneWiz box outside our lab. To use this box, select "UW Box A," the by-request box, so they know to pick up our samples. They don't come up to our box if nobody submitted a sample.

Preparing Samples

15 uL total including 5 uL of 5 uM primers.
- Keep a fresh stock of 5 uM primers that you take good care of (keep clean) and replace often with fresh stock.

Red Flags:
- Low concentration minipreps (<70 ng/uL) frequently fail when submitted to sequencing. It may be due to impurities that co-elute; if you submit many uL of this to meet the 500 ng/sample requirement, then you will have more of these impurities present. -Janet 3/20/2012

Sequencing Un-Purified PCR products

Submit 10 uL of PCR product and 5 uL of 5uM primer in a separate tube.
Best to submit a printed picture of the gel, too.
Submitting un-purified product costs ~$3/sample extra.
pmol/uL = uM

Sequencing Colonies

Submit 5uM primer in a separate tube and a plate with colonies.
Circle and number colonies you want sequence (I do this because I'll replica plate the ones I'm sending) or you can ask them to pick a variety.
Submitting costs ~$3/sample extra.

Order Submission Deadline

The cutoff time for sequencing is 4PM.
You can submit samples to the box a little after 4PM as long as you electronically submitted your order by 4PM. We are one of the last pickup sites so it takes a while for the person to get to our box.

Dropping of your samples to the Lab

If you miss the deadline, you can drop off samples at 1551 Eastlake Avenue E. They are on the first floor.

When Sequencing Fails

There are several ways it can fail & you can see the GeneWiz help for causes/solutions below. You can also watch this GeneWiz webinar. Don't hesitate to call GeneWiz customer support -- their customer service is incredible.
GeneWiz has very high standards for passing sequencing reactions. About 1/2 of your attempts may fail. Sometimes you can look at the trace file and decide it is good enough on your own despite a failed label.

Non-specific

- multiple are present on your DNA or you accidentally have a mixture of DNA templates.
  - You can prepare a new miniprep, with the hope that your first one was contaminated with another plasmid. Otherwise, you have to assume the plasmid you built accidentally contains an extra priming site. Of course, miniprepping from single colonies will reduce the possibility of mixed templates.
  - Note: a plasmid can contain an extra priming site via pcr/assembly fluke OR the insert you add can contain a mispriming site.
- hairpin present
- The clone has multiple priming sites (can be on accident)

Poor quality

high background: there is a clear sequence but there is also a background sequence.
- remnants of chromosomal DNA
- primer degradation: recall that your sequencing is dependent on length. So if you have one population of primers that is 20 bp and one that is 18 bp, they will give two separate signals.
top heavy: beginning sequence is strong; peaks may even be cut off. As it gets longer, the signal dies off. This is due to improper primer:template ratio; your primer may be "used up".

No priming:

lots of "N"s in sequencing result
- too much, too little, or no DNA
- no primer or sub-optimal primer concentration
- primer site not complementary
- carry-over inhibitors in the reaction such as phenol, ethanol, EDTA, or salts

Early termination

hairpin present, repetitive sequence, or high GC content can terminate the rxn sequencing. Note: they have several "difficult sequencing" protocols that can be used; select them in the form.
too much DNA
- results in smears. They can dilute the sample you sent and re-run it. Use 10ng/uL/kb of DNA.
bubble in capillary
- can appear as a smear. You won't know when this happens, but customer support may be able to tell.
dye blobs
- too many terminating nucleotides remain after their purification -- see image on right. A big peak covers the sequence you want. They generally have it at the beginning, so you should start your priming ~ 100 bp away from the sequence of interest. They happen on PCR products and plasmid & are best visually edited (ignored.)

High Background

what is the difference between High Background & non-specific?
- Customer support says: the degree to which the background sequence
- you can trust a sequence that fails because of high background more than you can non-specific

When it fails, try again!

You can submit 2 samples per order for a free repeat, but they must be on the same templates you submitted.
You can resequence as many as you like for 1/2 price and you have the choice to use new preps. This allows you to use a fresh miniprep or primer batch. If you want to submit fresh samples for 1/2 price, you should contact customer service and get approval. Write in the comments section at the bottom which samples are 1/2 price repeats, and which row & order the original failed sequence was in. Then call them with the order number for this new request/order. Janet 7/18/2012
Whether or not your repeat will be successful depends on several variables such as:
- the concentration and quality of the sample -- if a "no priming" or "poor quality" samples is "no priming" or "poor quality" after you sequence again, the quality and quantity might be too bad to work the 2nd time.
- you also may have a GC-rich region, hairpin or general difficult template that is causing binding issues, a problem with the binding site, a problem with the primer, etc.

Vague primer design instructions

"We recommend designing your sequencing primers in a region that is 100 bases upstream of your sequence of interest. If you do not have the luxury of having this buffer, the closest you want the primer to be to your area of interest is 50-60 bases. Anything closer and you risk missing a portion of your area of interest. The primers should be about 18-24 bases in length with a Tm of 56-60 degrees. The GC content should be about 45-55%. Many vendors that provide oligo synthesis services have software into which you can plug your primer sequence to check for Tm, GC content and homodimerization. For the oligo purity, desalting is all that is needed for sequencing" (link)
- Note that Finnzymes reports Tm higher than other calculators, so 62-65oC is probably good if using a Finnzyme calculation.

Sequencing un-purified PCR products

chose "custom" for the type of sequencing reaction
you can leave the DNA concentration field blank
- you can't do nano drop on DNA that hasn't been cleaned up (says customer service 1/2014) so you would have to compare it to a known concentration of ladder anyway.
pmol/uL [=] uM
include a photo of your gel in with the sequencing form.
It costs ~$3 more per reaction.
You can submit OneTaq 2X products, even though it has loading dye in it.

Sequencing gel purified PCR products

Organic solvents inhibit/inactivate the Taq used in Sanger sequencing.

Tip sent by technical support to Janet 5/2013:

Tips for Column Purification of Template DNA
- Here are a few guidelines to help aid in the effective column purification of your product.
- This will help to eliminate carry over of ethanol into the eluate.

Prior to elution, there is a wash step that includes a high concentration of ethanol. If you are using a micro spin column, after the wash step, please spin samples at maximum speed in the microfuge 2 times for 2 minutes decanting the flow through completely after the first spin and placing the column in a fresh tube for elution after the second spin.
If there is a rim around the membrane, carefully remove residual ethanol using a pipette tip after the second spin and then let the column sit for 2 minutes on the bench top prior to elution in order to promote residual ethanol evaporation.
Carefully elute with EB or water heated to 50'C by adding drop wise to the membrane surface. (I usually let this sit a couple min before spinning -ALS)
Spin at maximum speed for two minutes.

Please check your 260/280 and 260/230 ratios prior to sending samples for sequencing.
- The 260/230 ratio is very important since small deviations reflect contamination with organic solvents that essentially deactivate the taq and preclude informative sequencing results.

FAQs

FAQs

@@ Line 1: / Line 1: @@
-Return to [[Lidstrom:Protocols|Protocols]]
+Back to [[Lidstrom:Protocols|Protocols]]
-==Submitting Samples==
+Price per rxn: $6  [[User:Janet B. Matsen|JM 10/2012]]
-*Using the correct template mass and primer concentrations is crucial.  If you submit less than the recommended ng of DNA, sequencing fails more often.
+* This is the standard UW price, but volume discounts are possible if our lab starts using more.
-*If you have a low concentration plasmid prep, you can increase the mass you send by sending 0.5 uL of 100 uM primers (the stock concentration) instead of 5 uL of 5 uM primers.
-*The form has a section for notes.  The notes you can enter are for you only, not the sequencing center.  If you want to communicate with the sequencing staff, put it in the comments box at the bottom.  [[User:Janet B. Matsen|Janet]] 2/22/12
-==Aligning/Understanding Results==
+== SUBMIT TO UW By REQUEST Box A ==
-*[[User:Janet B. Matsen|Janet]] recommends doing a multiple alignment in NCBI's Blast webpage.  Do not use the APE program's aligner, especially if you have a repetitive sequence.  In Blast, try varying stringency for the match criteria if you don't have perfect alignment or you don't align the whole sequencing read to your expected sequence.
+* In summer of 2013 we got a GeneWiz box outside our lab.  To use this box, select "UW Box A," the by-request box, so they know to pick up our samples.  They don't come up to our box if nobody submitted a sample.
-**If you get an imperfect match or fail to match to your expected sequence, you can loosen the stringency requirements by selecting "somewhat dissimilar" or "more dissimilar" instead of "highly similar."
-**Always have good labels in your FASTA files to make sure you don't mix things up.
+==Preparing Samples==
-**If you are making variants of a construct, you can compare your sequencing results to all of the things you are making.  First make a text document with each of the reference sequences you are creating by pasting them back to back in a text editor.  Include descriptions for each e.g. "> SH3-FLS in pSB1A3".  Paste your sequence from GeneWiz into the top box and all of the other sequences in the bottom box.  When the results are returned, click the "max score" button & it will put the match with the highest score first.  This is most likely your product, but a sequencing read can match to multiple designs depending on your project.
+*15 uL total including 5 uL of 5 uM primers.
+**Keep a fresh stock of 5 uM primers that you take good care of (keep clean) and replace often with fresh stock.
+[[image:GeneWiz sample submission guideline.jpg|thumb|upright=1.9|center|GeneWiz sample submission guideline]]
+*Red Flags:
+**Low concentration minipreps (<70 ng/uL) frequently fail when submitted to sequencing.  It may be due to impurities that co-elute; if you submit many uL of this to meet the 500 ng/sample requirement, then you will have more of these impurities present.   -[[User:Janet B. Matsen|Janet 3/20/2012]]
+=== Sequencing Un-Purified PCR products ===
+* Submit 10 uL of PCR product and 5 uL of 5uM primer in a '''separate''' tube.
+* Best to submit a printed picture of the gel, too.
+* Submitting un-purified product costs ~$3/sample extra.
+* pmol/uL = uM
+=== Sequencing Colonies ===
+* Submit 5uM primer in a '''separate''' tube and a plate with colonies.
+* Circle and number colonies you want sequence (I do this because I'll replica plate the ones I'm sending) or you can ask them to pick a variety.
+* Submitting costs ~$3/sample extra.
+== Order Submission Deadline ==
+* The cutoff time for sequencing is 4PM.
+* You can submit samples to the box a little after 4PM as long as you electronically submitted your order by 4PM.  We are one of the last pickup sites so it takes a while for the person to get to our box.
+== Dropping of your samples to the Lab ==
+If you miss the deadline, you can drop off samples at [https://www.google.com/maps/place/1551+Eastlake+Ave+E/@47.633399,-122.326322,17z/data=!3m1!4b1!4m2!3m1!1s0x54901521431b5d01:0xdfaa192e0856f09e 1551 Eastlake Avenue E.]
+They are on the first floor.
 ==When Sequencing Fails==
-*There are several ways it can fail & you can see the GeneWiz help for causes/solutions below.
+*There are several ways it can fail & you can see the GeneWiz help for causes/solutions below.  You can also watch this [http://www.genewiz.com/file/dnaseq201/dnaseq201.html GeneWiz webinar].  Don't hesitate to call GeneWiz customer support -- their customer service is incredible.
-**[https://clims3.genewiz.com/Customer/Support/Troubleshooting/Non-Specific.pdf Non-specific]
+*GeneWiz has very high standards for passing sequencing reactions.  About 1/2 of your attempts may fail.  Sometimes you can look at the trace file and decide it is good enough on your own despite a failed label.
-**[https://clims3.genewiz.com/Customer/Support/Troubleshooting/Poor%20Quality.pdf Poor quality]
-**[https://clims3.genewiz.com/Customer/Support/Troubleshooting/No%20Priming.pdf No priming]
+===[https://clims3.genewiz.com/Customer/Support/Troubleshooting/Non-Specific.pdf Non-specific]===
+**multiple are present on your DNA or you accidentally have a mixture of DNA templates.
+***You can prepare a new miniprep, with the hope that your first one was contaminated with another plasmid.  Otherwise, you have to assume the plasmid you built accidentally contains an extra priming site.  Of course, miniprepping from single colonies will reduce the possibility of mixed templates.
+***Note: a plasmid can contain an extra priming site via pcr/assembly fluke OR the insert you add can contain a mispriming site.
+**hairpin present
+**The clone has multiple priming sites (can be on accident)
+===[https://clims3.genewiz.com/Customer/Support/Troubleshooting/Poor%20Quality.pdf Poor quality] ===
+*high background: there is a clear sequence but there is also a background sequence.
+**remnants of chromosomal DNA
+**primer degradation: recall that your sequencing is dependent on length.  So if you have one population of primers that is 20 bp and one that is 18 bp, they will give two separate signals.
+*top heavy: beginning sequence is strong; peaks may even be cut off.  As it gets longer, the signal dies off.  This is due to improper primer:template ratio; your primer may be "used up".
+===[https://clims3.genewiz.com/Customer/Support/Troubleshooting/No%20Priming.pdf No priming]:  ===
+*lots of "N"s in sequencing result
+**too much, too little, or no DNA
+**no primer or sub-optimal primer concentration
+**primer site not complementary
+**carry-over inhibitors in the reaction such as phenol, ethanol, EDTA, or salts
+===[https://clims3.genewiz.com/Customer/Support/Troubleshooting/Early%20Termination.pdf Early termination]===
+*hairpin present, repetitive sequence, or high GC content can terminate the rxn sequencing.  Note: they have several "difficult sequencing" protocols that can be used; select them in the form.
+*too much DNA
+**results in smears.  They can dilute the sample you sent and re-run it. Use 10ng/uL/kb of DNA. [[image:GeneWiz - Too Much DNA.png|thumb]]
+*bubble in capillary
+**can appear as a smear.  You won't know when this happens, but customer support may be able to tell.
+*dye blobs [[image:dye_blob_GeneWiz.png|thumb]]
+**too many terminating nucleotides remain after their purification -- see image on right.  A big peak covers the sequence you want.  They generally have it at the beginning, so you should start your priming ~ 100 bp away from the sequence of interest.  They happen on PCR products and plasmid & are best visually edited (ignored.)
+===[https://clims3.genewiz.com/Customer/Support/Troubleshooting/High%20Background.pdf High Background]===
+* what is the difference between High Background & non-specific?
+** Customer support says: the degree to which the background sequence
+** you can trust a sequence that fails because of high background more than you can non-specific
+=== When it fails, try again! ===
 *You can submit 2 samples per order for a free repeat, but they must be on the same templates you submitted.
-*You can resequence as many as you like for 1/2 price and you have the choice to use new preps.  This allows you to use a fresh miniprep or primer batch.  If you want to submit fresh samples for 1/2 price, you may want to contact customer service and get approval.  Once I put in a new order and note which are free repeats, and their respective order number in the "Notes" section of the form and they told me that was ok, but I got mixed messages about this.  [[User:Janet B. Matsen|Janet 2/22/12]]
+*You can resequence as many as you like for 1/2 price and you have the choice to use new preps.  This allows you to use a fresh miniprep or primer batch.  If you want to submit fresh samples for 1/2 price, you should contact customer service and get approval.  Write in the comments section at the bottom which samples are 1/2 price repeats, and which row & order the original failed sequence was in.  Then call them with the order number for this new request/order. [[User:Janet B. Matsen|Janet 7/18/2012]]
-**If you need to sequence another 1/2 price rxn, you should probably chat with customer service and they will put a note on the account.  They usually tell you to put the name of who you chatted with on the form, too.
 *Whether or not your repeat will be successful depends on several variables such as:
 **the concentration and quality of the sample -- if a "no priming" or "poor quality" samples is "no priming" or "poor quality" after you sequence again, the quality and quantity might be too bad to work the 2nd time.
 **you also may have a GC-rich region, hairpin or general difficult template that is causing binding issues, a problem with the binding site, a problem with the primer, etc.
-== Miscellaneous ==
+== Vague primer design instructions ==
-*Will my sequences be online forever?
+*"We recommend designing your sequencing primers in a region that is 100 bases upstream of your sequence of interest. If you do not have the luxury of having this buffer, the closest you want the primer to be to your area of interest is 50-60 bases. Anything closer and you risk missing a portion of your area of interest. The primers should be about 18-24 bases in length with a Tm of 56-60 degrees. The GC content should be about 45-55%. Many vendors that provide oligo synthesis services have software into which you can plug your primer sequence to check for Tm, GC content and homodimerization. For the oligo purity, desalting is all that is needed for sequencing" ([http://www.genewiz.com/public/DNA-sequencing-FAQs.aspx link])
-**Customer service: After three months, the data from your account will automatically be archived. If you would like the data for orders older than three months you may request a transfer of results back into your account.  All you would need to do is log into your account, go to "Order Status & Results", change the search conditions, select the orders you would like transferred by checking the box under the Transfer column and then hit the Transfer button. This will then automatically send our technical support department your request. You should be able to click on the order number an view the DNA names/primers; however, you won't have access to the trace files or sequences until you request that they are transferred back to your account.  -[[User:Janet B. Matsen|Janet]] 2/22/12 (from customer service chat)
+** Note that Finnzymes reports Tm higher than other calculators, so 62-65oC is probably good if using a Finnzyme calculation.
+== Sequencing un-purified PCR products ==
+* chose "custom" for the type of sequencing reaction
+* you can leave the DNA concentration field blank
+** you can't do nano drop on DNA that hasn't been cleaned up (says customer service 1/2014) so you would have to compare it to a known concentration of ladder anyway.
+* pmol/uL [=] uM
+* include a photo of your gel in with the sequencing form.
+* It costs ~$3 more per reaction.
+* You can submit OneTaq 2X products, even though it has loading dye in it.
-*Why don't they have VF2 and VR (the standard BioBrick primers) available at GeneWiz like they do for other common primers?
+== Sequencing gel purified PCR products ==
-**Janet (and others) have been lobbying for them to include these.  Stay tuned!  -[[User:Janet B. Matsen|Janet]] 2/22/12
+Organic solvents inhibit/inactivate the Taq used in Sanger sequencing.
+=== Tip sent by technical support to Janet 5/2013: ===
+* Tips for Column Purification of Template DNA
+** Here are a few guidelines to help aid in the effective column purification of your product.
+**This will help to eliminate carry over of ethanol into the eluate.
+# Prior to elution, there is a wash step that includes a high concentration of ethanol. If you are using a micro spin column, after the wash step, please spin samples at maximum speed in the microfuge 2 times for 2 minutes decanting the flow through completely after the first spin and placing the column in a fresh tube for elution after the second spin.
+# If there is a rim around the membrane, carefully remove residual ethanol using a pipette tip after the second spin and then let the column sit for 2 minutes on the bench top prior to elution in order to promote residual ethanol evaporation.
+# Carefully elute with EB or water heated to 50'C by adding drop wise to the membrane surface. (I usually let this sit a couple min before spinning -ALS)
+# Spin at maximum speed for two minutes.
+*Please check your 260/280 and 260/230 ratios prior to sending samples for sequencing.
+** The 260/230 ratio is very important since small deviations reflect contamination with organic solvents that essentially deactivate the taq and preclude informative sequencing results.
-*How much does each reaction cost?
+==FAQs==
-**Our lab pays $6/rxn if sequencing 1-47 samples in an order OR $5/rxn if 48 or more samples are sequenced per order.  Some labs that sequence much more frequently (e.g. David Baker) pay $1.50/sequence less because of their volume.
+*[http://www.genewiz.com/public/DNA-sequencing-FAQs.aspx FAQs]