We present a method of targeted ancient DNA sequence retrieval, which we used to reconstruct the complete mitochondrial genomes of five Neandertal individuals. Comparison of these sequences with present day humans suggests that Neandertals had a long term low effective population size.
This method was used in the research reported in Briggs et al., Science 325 (5938). 318-321 (2009).
Reagents required:
For manufacturer information regarding non-standard reagents and equipment see later table.
1) Library amplification
Reagent | μl per reaction |
Water | 45 |
10X Gene Amp PCR buffer II | 10 |
MgCl2 (25mM) | 10 |
BSA (10 mg / ml) | 2 |
dNTPs (25 mM each) | 1 |
454 emPCR fwd primer/10uM | 3 |
454 emPCR rvs primer/10uM | 3 |
AmpliTaq Gold DNA polymerase (5 U / μl) | 1 |
454 DNA library template | 25 |
Total | 100 |
2 ) Primer Extension
Reagent | μl per reaction |
Water | 45 |
10X Gene Amp PCR buffer II | 10 |
MgCl2 (25mM) | 10 |
BSA (10 mg / ml) | 2 |
dNTPs (25 mM each) | 1 |
454 emPCR fwd primer/10uM | 3 |
454 emPCR rvs primer/10uM | 3 |
AmpliTaq Gold DNA polymerase (5 U / μl) | 1 |
454 DNA library template | 25 |
Total | 100 |
3) Extension Product Capture
4) Capture Product Amplification
Reagent | μl per reaction |
Water | 45 |
10X Gene Amp PCR buffer II | 10 |
MgCl2 (25mM) | 10 |
BSA (10 mg / ml) | 2 |
dNTPs (25 mM each) | 1 |
454 emPCR fwd primer/10uM | 3 |
454 emPCR rvs primer/10uM | 3 |
AmpliTaq Gold DNA polymerase (5 U / μl) | 1 |
Eluted capture product | 25 |
Total | 100 |
Representative Results:
It is strongly recommended when starting out with the PEC protocol to perform first a capture reaction where a small amount of a ‘positive control target sequence’ (e.g. a ~100bp PCR product – 1 picogram is easily enough) is mixed in with the normal recommended amount of amplified 454 library template (see step 2.1), and capture is performed with a single PEC primer designed to capture the positive control product. If this control reaction is performed, qPCR with both positive control-specific and 454 adaptor-specific primer pairs can be used to quantify the amount of ‘control target’ versus background in the purified primer extension reaction (1.3), primer extension product (2.3) and eluted bead capture product (3.6). In this way, both the effectiveness of background removal (“specificity”) and the efficiency of target recovery (“sensitivity”) in your experimental conditions can be directly measured.
A successful PEC protocol normally has the following properties –
Sensitivity (measured by amount of control target retained through the protocol):
Total amount of control target in eluted bead capture product (3.6) =~ 1-20% of total amount in purified primer extension reaction (2.3).
Background (measured by 454 emPCR primer pair):
Total amount of background in eluted bead capture product (3.6) < 0.01% of total amount in purified primer extension reaction (2.3).
If there is less than 1% of the target remaining in the final product, the primer extension step may have been unsuccessful and should be investigated.
If there is much more than 0.01% of the background remaining in the final products, the washing steps may have been incorrectly performed and should be investigated.
The PEC method is simple, quick, sensitive and specific. Therefore we the authors envisage multiple applications outside ancient DNA, such as capture of small RNA fragments from an RNA library, interrogation of structural variation in a pooled sample or capture of 16S (or other loci) diversity from a metagenomic sample. One point to mention is that the sensitivity of capture becomes lower as the number of PEC primers in a multiplex capture reaction increases. PEC is therefore not ideally suited for capture of very large (e.g. a megabase or more) capture regions, but is extremely well suited for capture of small target regions or even SNP positions from many individuals in a rapid fashion.
The authors have nothing to disclose.
We thank M. Meyer for advice; The Croatian Academy of Sciences and Arts and the Berlin-Brandenburg Academy of Sciences for logistic and scientific support; and the Presidential Innovation Fund of the Max Planck Society for financial support. J.M.G. was supported by an NSF international postdoctoral fellowship (OISE-0754461). Sequences are deposited at the EBI nucleotide database with accession numbers: Neandertal 1 (Feldhofer 1) FM865407, Neandertal 2 (Feldhofer 2) FM865408, Sidron 1253 FM865409, Vindija 33.25 FM865410, Mezmaiskaya 1 FM865411
Material Name | Tipo | Company | Catalogue Number | Comment |
---|---|---|---|---|
AmpliTaq Gold polymerase with GeneAmp PCR buffer II and MgCl2 | Applied Biosystems | N8080241 | ||
QIAGEN MinElute PCR purification kit | Qiagen | 28004 | ||
M-270 streptavidin beads | Invitrogen | 653.05 | ||
Tween-20 | Sigma-Aldrich | P2287 | ||
DynaMag-2 magnetic particle separator | Invitrogen | 120.02D |