BioMicroCenter:Illumina Library Preparation: Difference between revisions

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[[Image:Presentationbest.jpg|right|400px]]
[[Image:BMC_samplePrep_pipes.png|thumb|right|400px|Sample Preparation available in BioMicro]]
Generating high quality data on the Illumina sequencing platform begins with generating high quality libraries that have the desired insert size, required Illumina adapters, and pass the BioMicro Center’s [[BioMicroCenter:Sequencing_Quality_Control|Sequencing Quality Control]] process. The BMC currently offers genomic DNA library preparation as a service; RNA-seq is being tested in beta.  
Generating high-quality data on the Illumina sequencing platform requires high-quality libraries. The BMC currently offers library preparation services for a variety of starting materials. Prior to sequencing, all samples must pass the BioMicro Center’s [[BioMicroCenter:Sequencing_Quality_Control|Sequencing Quality Control]] process, which verifies selection of inserts of a desired size and correct ligation of Illumina adapters.<br>Sample Prep questions can be directed to [[BioMicroCenter:People|Jon Penterman]].
==Sample Submission==
==Sample Prep Services==
There are two options when submitting samples for library prep:
Please follow the links in the table below for more information about our library preparation offerings.


'''BMC Illumina sample prep''' - Samples will be QC'd,  run on the SPRI-works system using BMC stored adapters, enriched using BMC stored PCR primers, and submitted for sequencing on the Illumina platform.
{| border=1
! DNA
! RNA
|-
| '''[[BioMicroCenter:DNA_LIB|Standard DNA Methods include]]'''
* LMPCR methods
** [[BioMicroCenter:DNA_LIB#SPRI_WORK|SPRI-works]]
** [[BioMicroCenter:DNA_LIB#NEOPREP|NeoPrep]]
* Tagmentation Methods
** [[BioMicroCenter:DNA_LIB#NEXTERA_.2F_NEXTERAXT|Nextera / NexteraXT]]


'''[[BioMicroCenter:SPRI-Works|SPRI-Works Direct Submission]]-''' - Samples will be run on the SPRI-works system using '''user supplied''' adapter mix and then returned for enrichment. If using this option please note that samples will need to be submitted separately for Illumina sequencing.
| '''[[BioMicroCenter:RNA_LIB|Standard RNA Methods include]]'''
* [[BioMicroCenter:#Illumina_TruSeq.2F_.7CNEOPREP|Illumina TruSeq done by Neoprep or by hand]]
* [[BioMicroCenter:RNA_LIB#EpiCenter_RiboZero|RiboZero]]
* [[BioMicroCenter:RNA_LIB#Clontech_SMARTer_Low-Input|Clontech v4 SMARTseq]]
* [[BioMicroCenter:RNA_LIB#NuGEN_Ovation_RNAseq_System_V2|Nugen Ovation v2]]
* NEB smallRNA prep
|-
| '''[[BioMicroCenter:DNA_HTL|High Throuhgput DNA Methods include]]'''
* Amplicon / 16S
* NexteraXT
* low input NexteraXT ''(coming soon)''
| '''[[BioMicroCenter:RNA_HTL|High Throuhgput RNA Methods include]]'''
* High Throughput 3' Digital Gene Expression (HT3DGE)
|}


==Sample Submission Requirements==
== OTHER SERVICES ===
'''Genomic DNA'''– At least 1ug of fragmented DNA is required.  It is recommended to fragment samples so the majority of the distribution is between 100 to 300bp.
=== [[BioMicroCenter:ChIP|ChromatinIP]] ===


'''RNA-Seq – Submission of total RNA samples for RNA-Seq is currently in early stages of beta testing. ''' RNA-Seq samples that have been mRNA selected, fragmented, and synthesized into dsDNA will be accepted for further library preparation.
'''ChIP-Seq''': Sonicated chromatin will undergo IP on the IPstar. RNase A, Proteinase K, Phenol:Chloroform extraction and purification will be performed off of the instrument and submitted for QC on the [[BioMicroCenter:2100BioAnalyzer|BioAnalyzer]]. These ChIP samples may be picked up for qPCR or sent directly to [[BioMicroCenter:SPRI-Works|SPRI]] for library construction and sequencing (options are listed on submission forms). Users will be contacted if ChIP samples fail QC. These samples will not be submitted to SPRI-works but will be charged for the IP.
All samples submitted will be QC’d using the [[BioMicroCenter:2100BioAnalyzer|BioAnalyzer]] to confirm sufficient fragmentation and concentration.
<BR><BR>
[[BioMicroCenter:Forms#Downloads|Sample Submission Forms]]
Sonicated chromatin should be submitted at 5-7 million cells per 200uL volume. Antibodies must be submitted at the same time(at least 3ug of antibody per IP). Chromatin should be prepared on the SAME DAY as the ChIP whenever possible. Full details about isolation methods can be found on the [[BioMicroCenter:ChIP|chromatin IP page]].


==Illumina Library Preparation Workflow==
=== SIZE SELECTION ===
[[Image: Libprep3.jpg|right|450px]]
The BMC offers [[BioMicroCenter:PippinPrep|PippinPrep Size Selection]] post library construction if custom insert sizes are needed.
*Fragmentation - All samples must be fragmented to the point where the majority of the fragment distribution is between 100 to 300 base pairs. RNA-seq samples are usually fragmented after poly-A selection and before first strand synthesis.
 
*End Repair and 3’ dA Addition – Any damage end damage that may have occurred during fragmentation is repaired and then an extra A is added to all 3’ ends to increase efficiency during ligation.  
== Barcoding ==
*Adapter ligation – The ligation of partial Illumina adapter sequence to the sample fragments, a total addition of 66bp. Each adapter sequence has a T overhang to increase efficiency. It is very important to maintain a good ratio of sample material to adapter, Illumina recommends a 1:10 ratio, to avoid primer dimmer occurrences post enrichment.
All library preparation service include indexing. [[BioMicroCenter:Multiplex|Molecular barcoding]] - identifying individual molecules from library preparation is available on [[BioMicroCenter:DNA_LIB|SPRIworks]] and as part of [[BioMicroCenter:RNA_HTL|HT3DGE]].
*Size Selection – This step, usually consisting of an agarose gel, is designed so that only the fragments within the desired size range (now ~200 – 400bp) are included in the final library.  Size selection is very important, fragments that are too large will create large clusters and can result in a loss of read count in the final data.  
 
*Enrichment – The PCR reaction run during this step amplifies using the complete primer construct required for binding and clustering on the flowcell, an addition of 53bp for a final adapter length of 119bpIt is very important to optimize the number of PCR cycles to generate a sufficient amount of material for clustering but limit PCR biases.
==Submission==
Traditional Illumina protocols can be found on our [[BioMicroCenter:Protocols| protocols page]]
Unless otherwise instructed, the BMC reserves 50% of submitted DNA in case of failures during sample prep. If you would like us to utilize the full sample, please indicate it in the notes section. <br><br>
 
'''DNA'''– DNA samples must be submitted in either water or TE. Although the [[BioMicroCenter:SPRI-Works|SPRIworks]] robot is not highly sensitive to the amount of DNA input, care must be taken to submit an [[BioMicroCenter:SPRI-Works|appropriate amount of '''adapter''' to ensure efficient ligation]]. If you select the Nextera kit instead of the SPRIworks, we will require 50ng of DNA input. If PCR products are submitted for Nextera prep, we recommend purifying the material prior to submission for best results.
   
'''RNA''' – Total RNA samples must be submitted in water or TE. The quantity of total RNA needs to be between 0.1-4ug for Illumina TruSeq, 1ug-4ug for strand specific RNAseq, >100pg for Low Input RNAseq.  


==High Throughput Library Preparation==
[[Image: BioMicro_SPRIworks.jpg|right|150px]]
The BMC is currently testing the Beckman SPRIworks library preparation system.  This platform is a fully automated library preparation system for Illumina sequencing and supports all Illumina applications except for smallRNA-Seq. It performs all of the traditional Illumina protocol steps listed above, except for Enrichment, and utilizes SPRI beads for size selection.  For more information on the SPRIworks platform please visit http://www.spriworks.com/.


== Pricing ==
Priority for Illumina sample prep is currently available for labs associated with the BioMicro Center [[BioMicroCenter:CoreDeps|Core departments]]. We are able to do Illumina sample prep for other MIT and [[BioMicroCenter:FAQ#NON_MIT_USERS|non-MIT]] users as space allows on the sequencers. Full pricing information is available at [[BioMicroCenter:Pricing|our price list]].


== Protocols ==
'''[[BioMicroCenter:Forms#Downloads|Sample Submission Forms]]'''<br><br><br>
Protocols for all of the supported technologies can be found by visiting the [[BioMicroCenter:Protocols| Protocols]] page


== QC ==
== QC ==


Quality control is very important to help optimize the number of reads and quality of data produced. For information on QC methods and protocols please visit the [[BioMicroCenter:Sequencing_Quality_Control|Sequencing Quality Control]] page
Good quality control is crucial for optimizing the number of reads and quality of data produced by the sequencers. For more information on QC methods and protocols please visit the [[BioMicroCenter:Sequencing_Quality_Control|Sequencing Quality Control]] page. <br><br><br>
 
==Workflow==
[[Image: Libprep3.jpg|right|450px]]
* Fragmentation - All samples must be fragmented to the point where the majority of the fragment distribution is between 100 to 300 base pairs.  RNA-seq samples are usually fragmented after poly-A selection and before first strand synthesis.<br>
* End Repair and 3’ dA Addition – Any end damage that may have occurred during fragmentation is repaired and then an extra A is added to all 3’ ends to increase efficiency during ligation. <br>
* Adapter ligation – Partial Illumina adapter sequences are ligated to the sample fragments, a total addition of 66bp between the two ends. Each adapter sequence has a T-overhang to increase efficiency. It is very important to maintain a good ratio of sample material to adapter. Illumina recommends a 1:10 ratio, to avoid the presence of primer-dimer after enrichment.<br>
* Size Selection – This step is designed so that only the fragments within the desired size range (generally ~200–400bp) are included in the final library.  Size selection is very important: fragments that are too large will create oversized, overlapping clusters on the Illumina flowcell and can result in a loss of read count in the final data. Fragments much smaller than the optimal size range may include residual primers and primer-dimers. Size selection is usually performed using an agarose gel.<br>
* Enrichment – The DNA is PCR-amplified using the complete primer constructs required for binding and clustering on the flowcell. This adds 53bp of adapter sequence total between the two ends, for a final adapter length of 119bp.  It is very important to optimize the number of PCR cycles so that there is sufficient material for clustering while limiting PCR biases.<br>
 
Traditional Illumina protocols can be found on our [[BioMicroCenter:Protocols| protocols page]]. <br><br><br>
 
 
<br>
<br>
<br>
 


== Pricing and Priority ==
Full pricing information is available on [[BioMicroCenter:Pricing|our price list]].<br>


All questions about Illumina Sequencing can be directed to Ali Perrotta at aperrott@mit.edu.
Priority for Illumina sample prep is currently given to labs associated with the BioMicro Center [[BioMicroCenter:CoreDeps|Core departments]]. We are able offer our services to other MIT and [[BioMicroCenter:FAQ#NON_MIT_USERS|non-MIT]] users as space allows. <br><br><br>

Revision as of 07:49, 25 August 2016

HOME -- SEQUENCING -- LIBRARY PREP -- HIGH-THROUGHPUT -- COMPUTING -- OTHER TECHNOLOGY
Sample Preparation available in BioMicro

Generating high-quality data on the Illumina sequencing platform requires high-quality libraries. The BMC currently offers library preparation services for a variety of starting materials. Prior to sequencing, all samples must pass the BioMicro Center’s Sequencing Quality Control process, which verifies selection of inserts of a desired size and correct ligation of Illumina adapters.
Sample Prep questions can be directed to Jon Penterman.

Sample Prep Services

Please follow the links in the table below for more information about our library preparation offerings.

DNA RNA
Standard DNA Methods include Standard RNA Methods include
High Throuhgput DNA Methods include
  • Amplicon / 16S
  • NexteraXT
  • low input NexteraXT (coming soon)
 High Throuhgput RNA Methods include
  • High Throughput 3' Digital Gene Expression (HT3DGE)

OTHER SERVICES =

ChromatinIP

ChIP-Seq: Sonicated chromatin will undergo IP on the IPstar. RNase A, Proteinase K, Phenol:Chloroform extraction and purification will be performed off of the instrument and submitted for QC on the BioAnalyzer. These ChIP samples may be picked up for qPCR or sent directly to SPRI for library construction and sequencing (options are listed on submission forms). Users will be contacted if ChIP samples fail QC. These samples will not be submitted to SPRI-works but will be charged for the IP.

Sonicated chromatin should be submitted at 5-7 million cells per 200uL volume. Antibodies must be submitted at the same time(at least 3ug of antibody per IP). Chromatin should be prepared on the SAME DAY as the ChIP whenever possible. Full details about isolation methods can be found on the chromatin IP page.

SIZE SELECTION

The BMC offers PippinPrep Size Selection post library construction if custom insert sizes are needed.

Barcoding

All library preparation service include indexing. Molecular barcoding - identifying individual molecules from library preparation is available on SPRIworks and as part of HT3DGE.

Submission

Unless otherwise instructed, the BMC reserves 50% of submitted DNA in case of failures during sample prep. If you would like us to utilize the full sample, please indicate it in the notes section.

DNA– DNA samples must be submitted in either water or TE. Although the SPRIworks robot is not highly sensitive to the amount of DNA input, care must be taken to submit an appropriate amount of adapter to ensure efficient ligation. If you select the Nextera kit instead of the SPRIworks, we will require 50ng of DNA input. If PCR products are submitted for Nextera prep, we recommend purifying the material prior to submission for best results.

RNA – Total RNA samples must be submitted in water or TE. The quantity of total RNA needs to be between 0.1-4ug for Illumina TruSeq, 1ug-4ug for strand specific RNAseq, >100pg for Low Input RNAseq.


Sample Submission Forms


QC

Good quality control is crucial for optimizing the number of reads and quality of data produced by the sequencers. For more information on QC methods and protocols please visit the Sequencing Quality Control page.


Workflow

  • Fragmentation - All samples must be fragmented to the point where the majority of the fragment distribution is between 100 to 300 base pairs. RNA-seq samples are usually fragmented after poly-A selection and before first strand synthesis.
  • End Repair and 3’ dA Addition – Any end damage that may have occurred during fragmentation is repaired and then an extra A is added to all 3’ ends to increase efficiency during ligation.
  • Adapter ligation – Partial Illumina adapter sequences are ligated to the sample fragments, a total addition of 66bp between the two ends. Each adapter sequence has a T-overhang to increase efficiency. It is very important to maintain a good ratio of sample material to adapter. Illumina recommends a 1:10 ratio, to avoid the presence of primer-dimer after enrichment.
  • Size Selection – This step is designed so that only the fragments within the desired size range (generally ~200–400bp) are included in the final library. Size selection is very important: fragments that are too large will create oversized, overlapping clusters on the Illumina flowcell and can result in a loss of read count in the final data. Fragments much smaller than the optimal size range may include residual primers and primer-dimers. Size selection is usually performed using an agarose gel.
  • Enrichment – The DNA is PCR-amplified using the complete primer constructs required for binding and clustering on the flowcell. This adds 53bp of adapter sequence total between the two ends, for a final adapter length of 119bp. It is very important to optimize the number of PCR cycles so that there is sufficient material for clustering while limiting PCR biases.

Traditional Illumina protocols can be found on our protocols page.







Pricing and Priority

Full pricing information is available on our price list.

Priority for Illumina sample prep is currently given to labs associated with the BioMicro Center Core departments. We are able offer our services to other MIT and non-MIT users as space allows.


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