Double-SPRI (dSPRI) DNA fragment size-selection

High-molecular weight genomic DNA was obtained from a marine environmental sample (Hawaii Ocean Time Series, cruise 186, 75 m depth, [10]) and from laboratory cultures using standard procedures [14], or by amplifying genomes from individually flow-sorted cells as described [15]. DNA samples (50 µL, 2 µg) were sheared using 18–24 cycles of alternating 30 seconds ultasonic bursts and 30 seconds pauses in a 4°C water bath (Bioruptor UCD-200, Diagenode). The resulting DNA molecules were end-repaired and phosphorylated according to manufacturer's recommendations (End-repair kit, Enzymatics or New England Biolabs). The size distribution of the resulting fragments ranged on average from ∼100 to ∼700 bp as judged by Agilent Bioanalyzer DNA-1000 assays.

We optimized a two-step dSPRI protocol [4] for DNA fragment size selection that quantitatively removes fragments above or below the desired size range. In a first separation step, DNA fragments above an upper size threshold are bound by Agencourt AMPure XP SPRI magnetic beads and discarded. In the following second separation step fragments in the desired size range are selectively captured on the beads while all shorter fragments are discarded with the supernatant. The conditions during first and second separation are tunable to enable selective enrichment for other fragment size distributions (Figure 1). In addition, we showed that the size specificity of the dSPRI procedure is stable over a wide range of DNA concentrations (Figure 2). The sequencing libraries prepared for this work were obtained by combining 50 µL of sheared DNA with 40 µL of Agencourt AMPure XP SPRI magnetic beads and incubated at room temperature for 5–7 minutes. The tubes were next placed on a magnet holder (Invitrogen-Dynal) for 2 minutes before transferring the supernatant to a new tube and discarding AMPure XP particles from this first separation step. For the second separation step, 100 µL of fresh AMPure XP beads were added to 85 µL of the supernatant from the previous separation, mixed well, and incubated for 5 minutes before transferring the tube to the magnet holder rack. The supernatant from this second step was discarded and the SPRI particles were washed twice with 0.5 mL of 70% ethanol. The wash steps ensure complete removal of polyethylene glycol (PEG) and salts, but also of any remaining unbound fragments smaller than the desired fragment size distribution. After removing the 70% ethanol from the wash steps, the beads were air dried at room temperature (or at 37°C) for 10–15 minutes. In order to recover the bound DNA, 30 µL of water was added to the beads, and incubated at room temperature for at least 1 minute. The DNA solution was separated from the Agencourt AMPure XP SPRI magnetic beads for 2 min on the magnet holder, and transferred to a new tube. Applying aforementioned conditions for dSPRI led to the specific enrichment of a DNA size-fraction with an average size of 207 bp. Enrichment for other size distribution can easily be achieved by modifying the dSPRI conditions as described in Figure 1.

Illumina paired-end library construction

Our strategy to create Illumina compatible sequencing libraries uses a blunt-end ligation step of two distinct adapters rather than the ligation of a single Y-shaped adapter [16]. dSPRI-selected DNA fragments were combined with a 10-fold molecular excess for each oligonucleotide adapters (see Table 1 for oligonucleotide sequences). Blunt-end DNA fragments were ligated using a rapid-ligation kit (Enzymatics or New England Biolabs) for 5–10 minutes at room temperature. Adapter excess was subsequently removed using Agencourt AMPure XP SPRI beads according to the manufacturer's recommendations (DNA/bead ratio of 1). A nick-translation step was performed with 2 units of BstI exo^- DNA polymerase (New England Biolabs) at 65°C for 25 minutes in a reaction consisting of 20 mM Tris-HCl pH 8.8, 10 mM (NH₄)₂SO₄, 10 mM KCl, 2 mM MgSO₄, and 0.1% Triton X-100. The resulting DNA fragments were diluted 2 fold with ddH₂O, and PCR amplified using Phusion Hot Start High-Fidelity DNA polymerase (New England Biolabs), and simultaneously monitored on a Bio-Rad Opticon real-time PCR instrument. Each reaction consisted of 1 µL of diluted nick-translated DNA, 0.5 units of Phusion Hot Start High-Fidelity DNA polymerase, 1X Phusion HF buffer, 0.4 µM of each IGA-PCR-PE-F and IGA-PCR-PE-R primers [described in Table 1], 200 µM dNTPs as well as 0.25X SYBR green I. The initial denaturation step was at 98°C for 1 minute, followed by successive cycles of 98°C for 15 seconds, 65°C for 10 seconds and 72°C for 15 seconds. The reactions were stopped in the late logarithmic amplification phase, and the DNA from the corresponding samples were pooled. The resulting libraries were composed of fragments with distinct adapters at each extremities due to PCR suppression effect [17]–[19]. The amplified libraries were subjected to an additional round of AMPure XP SPRI beads purification, with a DNA/beads ratio of 1, to remove residual primers and adapter dimers.

In order to achieve optimal cluster densities for sequencing on the Illumina GAII platform, samples were quantified using two methods. The samples were first analyzed using the High-Sensitivity DNA Kit for the Bioanalyzer (Agilent Technologies) to detect any primer-dimers and to determine the average molecular weight of each library. The samples were next quantified by real-time PCR on a LightCycler II 480 (Roche), using the LightCycler 480 SYBR Green I Master mix (Roche), appropriate primers (Table 1), and serially diluted PhiX 335 bp control library (Illumina) as a standard (quantified with the Agilent Bioanalyzer; we observed that the Illumina PhiX 335 bp concentration vary from lot to lot, and typical concentrations were found to range from 11–15 nM). The phiX standard curve was required to have an r² value of >0.98 or the run was repeated. This step both confirmed the concentration of the libraries as well as confirmed the presence of proper primers for Illumina sequencing.

Illumina paired-end sequencing

Illumina libraries were clustered for sequencing immediately following sample quantification according to manufacturers recomendations (Illumina). Following clustering, the samples were loaded on to an Illumina GAIIx sequencer. Sequencing reagents for each read were pooled prior to loading. Data from the Illumina GAIIx was analyzed using the Illumina pipeline 1.4.0 to generate fastq files.

Mate-Read Overlapper Algorithm

In order to align overlapping mate reads and produce accurate composite fragments, we developed the SHERA software pacakge, a collection of computer code written in the PERL programming language. The algorithm for aligning paired reads and computing quality scores was designed to be broadly applicable, independent of the sequencing platform. The source code is freely available at http://almlab.mit.edu/ALM/Software/Software.html. In brief, SHERA takes overlapping short reads as input, finds the best alignment, produces a composite read, calculates new quality scores for the overlapping bases, and scores the alignment confidence. A detailed description of each of these steps is provided below. We also describe our procedure for evaluating false alignment rates on both real and simulated reads.

Finding the best alignment

For each mate-pair, the algorithm scores all possible ungapped alignments (this includes alignments shorter than the read length, which are produced when a fragment is fully sequenced resulting in and additional synthesis reactions proceed past its 5-prime end, base-pairing with the Illumina adapters.) Each alignment is scored by summing over all matches and subtracting a penalty for each mismatch. For the alignment with the best score, the algorithm constructs the consensus sequence in this overlapping region by reporting the nucleotide with the higher quality value, or the informative base call if one nucleotide is 'N'. A Phred quality score is calculated for each consensus base (see below). The algorithm output includes sequence and quality of the composite read generated from each mate pair, as well as an alignment confidence score that enables filtering out probable mis-alignments.

Alignment confidence metric

Alignment confidence was quantified in order to identify composite reads constructed from mis-alignments. Due to the relatively short alignment lengths with non-uniform base composition and quality, we did not model the statistical significance of an alignment analytically, but instead chose an empirical metric. Because mis-alignments of similar length have similar alignment scores (within noise), we use seven alignments of similar length of the same mate-pair to calculate a baseline, and divide by the range of the scores to estimate the alignment's significance. Alignments of all confidence levels are reported; we leave selection of this threshold to the user to achieve the sensitivity/specificity required of their downstream application.

Calculation of a Phred Quality Score for the overlapped region

SHERA reports a Phred-scaled error probability for each base in the composite read. For overlapped bases, this is the posterior probability that the consensus base is wrong, given the base calls at that position in the alignment and their respective quality scores. Calculating this probability required making a few assumptions and approximations:

1. Given a basecall was in error, there is a uniform probability of reporting one of the other three bases.
2. The probability of correct alignment was approximated to be 1. (A decent approximation given true-positive rates of >99% in our quality filtered alignments, see Counting False Alignments below).
3. The basecalls of the forward and reverse read are independent observations, given the true base in the insert.
4. The prior probability of a base being present in an insert in this flowcell can be estimated from the low-error portion of the reads or approximated as uniform at the user's discretion (In our case, we used empirical observations to estimate %GC in single-genome samples, and a uniform distribution for the metagenomic sample.)

We first confirmed that the posterior error probability for the overlapped region was correct by counting the true error rate in composite reads constructed from simulated reads. Next, using real mate-reads as input, we confirmed that our Phred quality scores up to 32 correspond to the correct error rate as calculated by comparing to the reference. Above 32, the error rate does not improve (for neither the overlapped bases nor the original Illumina bases). This is due to errors in the reference and/or a very small percentage of Illumina reads with insertions or deletions.

Counting False Alignments

Minimizing the number of false alignments is an important step for some applications such as de novo assembly. Our goal was to find a threshold for alignment confidence that would allow no more than 1% misalignments to remain in our subset of composite reads (based on previous experience with de novo assembly of libraries containing hybrid reads). We used several approaches to assess our alignment accuracy and found similar results.

First, we used the read-simulator from the MAQ package [20] to produce simulated reads that mimicked the error profiles observed in the quality values of our Illumina data as well as the distribution of overlap lengths. In the case of simulated reads, the true distance between mate pairs is known exactly and the reference is perfect. After filtering (confidence metric ≥0.5) we retain 89.7% of the composite reads, 0.5% of which were constructed from mis-alignments. This strategy is useful when no reference is available, or as a test case on new platforms.

Second, we used mate-reads from the PhiX control lane sequenced during our Illumina sequencing run. This DNA library is prepared from the PhiX174 bacteriophage genome for purposes of quality control, and we found that it had and insert length 200±21 bp (estimated by mapping to the reference with MAQ). These mapped mate-pairs defined the “true” insert length of each sequenced fragment. After constructing the composite sequences and filtering, we plotted the difference in length between a composite fragment and its insert length as predicted by MAQ (Figure 7). This histogram is a sum of two distributions, the overlapper software's misalignments (a broad gaussian) and a sharp peak of small (1–2 bp) indels. We examined gapped alignments to confirm this was the case and also found that many of the insertion or deletions occur in homopolymer runs. We used a simple linear model to infer the number of misalignments; this yielded a false positive rate of 1.0% for PhiX174.

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Figure 7. Short insertions and deletions in low-confidence composite Illumina reads.

Mate-reads from the control lane (PhiX174 bacteriophage genome) were used to assess false alignments introduced by the SHERA pipeline. After constructing the composite sequences and filtering, we plotted the difference in length (if any) between a composite fragment and its insert length as predicted by MAQ by mapping the original mate-pairs to the reference.This histogram is a sum of two distributions, the overlapper software's misalignments (a broad gaussian) and a sharp peak of small (1–2 bp) indels. We used a simple and conservative linear model to remove the indels and infer the number of misalignments.

https://doi.org/10.1371/journal.pone.0011840.g007

Finally, for Figure 3C, we assessed alignment yield and accuracy on mate-pair reads sequenced from a dSPRI library. This library was generated from a single Prochlorococcus cell (as described [15]), for which a draft copy of the genome (N50 = ∼7 Kb) was constructed independently by de novo assembly of 454-Titanium reads from the same DNA sample. We mapped the Illumina mate-paired reads to these 454-Titanium contigs to define the “true” insert length of each sequenced insert. A small fraction of mate-pairs (<5%) were unmapped or mapped to different contigs; these were excluded from further analysis. As in the case of PhiX174, there were a number of small indels evident in the comparison between reads and reference which were excluded from our statistic. We estimate that 0.5% of our high confidence set of composite reads were mis-alignments introduced by SHERA.

Comparison of 454-FLX and overlapped Illumina reads for metagenomic applications

To evaluate the suitability of overlapped Illumina for metagenomic analysis, we made a direct comparison to the Roche 454-FLX platform, currently the most commonly used sequencing platform for this application. We used sequencing data from the exact same marine metagenomic sample [10]. We asked whether reads from the two platforms were equally able to identify significant protein homology with known proteins for the purposes of taxonomic classification.

We obtained 6,339,825 mate-paired Illumina reads of length 143 ntds each with insert lengths shown in Figure 3. We joined the Illumina mate-pair reads with our algorithm and filtered the composite reads by alignment confidence, resulting in 4,830,552 high-confidence composite reads of length 180±40 bp. We analyzed both high-confidence and low-confidence sets of composite reads as described below. We also had access to 673,673 454-FLX reads of length 207±71 ntds available for comparison [10]. We blasted all 454-FLX reads and composite Illumina reads against the NCBI protein database nr [21] using translated nucleotide queries (blastx parameters -b 100 -v 100 -e 30 -Q 11 -F “m S”), and used the popular metagenomics software MEGAN [22] for downstream analysis. We compared the fraction of unassignable reads (due to lack of significant blast hit in the database) across four subsets of sequence data from the same sample, which were chosen to compare sequencing platforms and the effect of read length: high-confidence composite Illumina reads, low-confidence composite Illumina reads, a representative sample of our 454 reads (mean length 207 bp), a longer subset of our 454 reads (mean length 254 bp). For comparison purposes we used random samples of 50,000 reads each. We used the MEGAN parameters recommended by the authors [22] as suitable for comparing reads of different lengths (minscore = 35.0, minscorebylength = 0.35, toppercent = 10, minsupport = 1; the low minsupport value was chosen because some of the data subsets tested were necessarily small. We also tested the alternative parameter set with similar results: minscore = 40.0, toppercent = 10, minsupport = 5). In Figure 6A we show the fraction of DNA fragments for which MEGAN was able to assign to a known genome or taxon via significant protein homology. We show that composite Illumina reads from high-confidence alignments perform at least as well as reads obtained from 454-FLX. We also find that composite reads produced by alignments we designated as “low-confidence” have a very high fraction of unassignable reads, further proof of the ability of our algorithm to identify misalignments. Finally, we show results for 454-FLX reads of mean length 254 bp (range: 230–270 bp), more typical of datasets produced by the 454-FLX platform. The assignable read fraction is comparable.

Next we asked if the taxonomic classification was consistent across platforms. We used MEGAN [22] to classify all of the 454-FLX reads and an equal number of composite Illumina reads. Figure 6B shows the taxonomic classification is relatively invariant with respect to the sequencing technology chosen. We performed this analysis with two reasonable parameters sets (minscore = 35.0, minscorebylength = 0.35, toppercent = 10, minsupport = 5 OR minscore = 40.0, toppercent = 10,minsupport = 5) and observed equally good agreement in taxonomic classification across platforms.