Improved DNA Sequencing Accuracy and Detection of Heterozygous Alleles Using Manganese Citrate and Different Fluorescent Dye Terminators

doi:10.1101/gr.9.6.588

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Vol. 9, Issue 6, 588-595, June 1999

METHODS
Improved DNA Sequencing Accuracy and Detection of Heterozygous Alleles Using Manganese Citrate and Different Fluorescent Dye Terminators

Christopher Korch,¹^,³ and Harry Drabkin¹^,²

¹ University of Colorado Cancer Center (UCCC) DNA Sequencing and Analysis Core and ² Division of Medical Oncology, School of Medicine, University of Colorado Health Sciences Center, Denver, Colorado 80262 USA

ABSTRACT

Top
Abstract
Introduction
RESULTS
DISCUSSION
METHODS
References

The use of dideoxynucleotide triphosphates labeled with different fluorescent dyes (dye terminators) is the most versatilemethod for automated DNA sequencing. However, variation in peakheights reduces base-calling accuracy and limits heterozygousallele detection, favoring use of dye-labeled primers for thispurpose. We have discovered that the addition of a manganese saltto the PE Applied Biosystems dye-terminator sequencing kits overcomesthese limitations for the older rhodamine dyes as well as themore recent dichloro-rhodamine dyes (dRhodamine and BigDyes).Addition of manganese to reactions containing dRhodamine-baseddye terminators produced the highest base-calling accuracy. Thiscombination resulted in the most uniform electropherogram profiles,superior to those produced by BigDye terminators and publishedfor dye primers, and facilitated detection of heterozygousalleles.

	INTRODUCTION

Top Abstract Introduction RESULTS DISCUSSION METHODS References

The most versatile means of automated DNA sequencing uses dye terminators, which are dideoxynucleotide triphosphates (ddNTPs)labeled with different fluorescent dyes. This allows performingthe sequencing reactions simultaneously in a single tube and electrophoresingthe products in a single lane (Prober et al. 1987). However, thevariability in electropherogram peak heights reduces base-callingaccuracy and hinders heterozygous mutation detection. Alternatively,sequencing primers can be individually labeled and used in separatesequencing reactions to produce more even peak heights, but thisdemands a more cumbersome and expensive procedure (Rosenblum etal. 1997).

Thermostable Thermus aquaticus (Taq) DNA polymerase strongly discriminates against ddNTPs in a manner dependent on sequencecontext (Tabor and Richardson 1989, 1990, 1995). Tabor and Richardson(1995) identified and altered a specific amino acid residue inDNA polymerases responsible for this discrimination. Two thermostable,genetically engineered DNA polymerases incorporating this mutation(phenylalanine 667 to tyrosine; F667Y) are now commercially available $---$ AmpliTaqDNA polymerase FS from PE Applied Biosystems (PE/ABI; Foster City,CA) and Thermo Sequenase from Amersham Life Science (ArlingtonHeights, IL; Reeve and Fuller 1995; Samols et al. 1995; VanderHorn et al. 1997). Use of these mutant polymerases and dye-labeledprimers produces electropherograms with very similar peak heightsalong the entire length of the readable sequence (McDonald etal. 1995; Samols et al. 1995; Vander Horn et al. 1997). However,peak heights are considerably less uniform when using these DNApolymerases in dye-terminator sequencingreactions.

A common problem with ddNTPs labeled with rhodamine-based dyes occurs where a G follows an A. The size of the dye-labeledG peaks is reduced (i.e., "suppressed") to less than both theaverage height of G peaks and the height of the preceding A peakin the sequence trace. The G peak sometimes is obscured not onlyby these A peaks, but also by the peak following a suppressedG, which can be much taller than average. Although Parker et al.(1995, 1996) and Zakeri et al. (1998) have analyzed the contextdependency of peak height variations to improve data interpretations,this variability still limits the usefulness of the dye terminators.To improve base calling of automated fluorescent sequencing, PE/ABIhas developed two alternatives to the rhodamine-based dye-terminators:4,7-dichloro-rhodamine-based dyes (dRhodamine dyes) and energy-transfervariants of the dRhodamine dyes (BigDyes) (Lee et al. 1997; Rosenblumet al. 1997). Dideoxynucleotides labeled with these dyes showmore uniform peak heights and less G suppression (Rosenblum etal. 1997; Zakeri et al. 1998). However, these improvements toboth the DNA polymerases and the labeling dyes do not producesequencing results as uniform as those with dye-labeled primers(Rosenblum et al. 1997) or with the wild-type phage T7 DNA polymeraseand the mutant enzyme Sequenase 2.0 (Tabor and Richardson 1989;Ju et al. 1995).

We recently reported a significant improvement of automated cycle sequencing that uses addition of MnCit (an equimolar combinationof manganese chloride and the metal buffer, trisodium citrate)to rhodamine-based dye-terminator cycle-sequencing reactions containingmagnesium and the F667Y variant Taq DNA polymerases (Korch andDrabkin 1999). In the present report, we characterize the effectsof MnCit addition on all three fluorescent dye-terminator cycle-sequencingprocedures from PE/ABI. The uniformity of peak heights is dramaticallyimproved, especially for the rhodamine- and dRhodamine-based sequencingkits, and is applicable to all four PE/ABI sequencing instruments:models 373A, 373A XL, 377, and 377 XL. MnCit addition, togetherwith other modifications of the DNA-sequencing protocol, significantlyincreases base-calling accuracy at minimal cost. Furthermore,the addition of manganese improves the detection of heterozygousnucleotidedifferences.

	RESULTS

Top Abstract Introduction RESULTS DISCUSSION METHODS References

MnCit Improves Peak Height Uniformity with Rhodamine, dRhodamine, and BigDye DNA-Sequencing Kits

As described earlier, the addition of MnCit to a reaction containing 1.5-2.0 mM magnesium improved the uniformity of peakheights produced by AmpliTaq DNA polymerase FS with the standardrhodamine dye terminators (Korch and Drabkin 1999). Figure 1 comparesthe effect of adding optimal amounts of MnCit to DNA cycle-sequencingreactions based on the newer dye-terminator kits: dRhodamine andBigDye. Using the control primer and pGEM3Zf(+) DNA template includedin the sequencing kits, MnCit addition produced distinctly moreuniform peak heights with the dRhodamine kit as we showed earlierwith the rhodamine kit, whereas its addition to the BigDye kitshowed only a slight improvement of peak height uniformity. Theapparent reduction in peak height of the dRhodamine + MnCit resultsis relative to the abnormally strong T peak in the 5'-GATC-3'sequence near the primer, but not included in the electropherogrampanel in Figure 1 (also see below). Using the rhodamine kit inthe presence of 0.5 mM trisodium citrate, addition of differentmanganese salts (chloride, sulfate, and acetate) all producedcomparable improvements on peak height variability (data not shown).

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Figure 1 Addition of MnCit reduces peak height variations in DNA sequencing electropherograms produced using different PE/ABI dye-terminator sequencing kits. Shown are electropherograms of DNA-sequencing reactions utilizing ddNTPs labeled with dyes based on dRhodamine and BigDye. The pGEM3Zf(+) template and the primer ( $-$ 21/pUC or M13F) were either from the PE/ABI rhodamine dye terminator Ready Mix sequencing kit, which were dissolved in TE (BigDye ± 0.8 mM MnCit results), or prepared by us and dissolved in water (dRhodamine ± 0.3 mM MnCit results). The underlined region of nucleotides 300-310 illustrates how the presence of MnCit reduces the suppression of G peaks that follow A peaks.

Most earlier papers describing the effects of manganese on sequencing used the metal buffer trisodium isocitrate at concentrationsof 4-25 mM (Fuller 1989; Tabor and Richardson 1989, 1990, 1995;Kristensen et al. 1990; Zimmermann et al. 1990). We found thatboth citrate and isocitrate could be used, but the optimal concentrationswere ~0.5 mM using the DNA template and primer controls from thekits. The improvement by MnCit was optimal at equimolar ratiosof MnCl₂ and trisodium citrate (data not shown). From the relativeintensities of banding patterns in fluorescent gel images andthe sum of the average signal strengths for the bases, concentrations>2 mM trisodium citrate or 2.5 mM trisodium isocitrate inhibitedthe sequencing reactions (data not shown). This loss of "activity"was caused by chelation of the enzymatic cofactor Mg²⁺, as addition of 1 mM and 2 mM MgCl₂ to the reaction mixturesrestored activity. MnCit concentrations >1.0 mM also caused theunincorporated dye terminators to precipitate more easily andto be more difficult to remove from the reactions by ethanol precipitationprior to loading on gels (data not shown). MnCit concentrations<0.7 mM also inhibited incorporation of dye terminators (datanot shown), but (1) increasing the amount of DNA template, (2)increasing the number of cycles used in the sequencing reactions,(3) loading a larger portion of the sequencing reactions on thegel, or (4) a combination of these measures could compensate forthese smaller losses of signalstrength.

The effect of increasing amounts of MnCit on profile variations was quantified by measuring the height of 100 consecutivepeaks. We found that increasing MnCit concentrations from 0.1mM to 1.0 mM decreased peak height variation sharply (as measuredby the coefficient of variation, CV, of peak heights, Fig. 2).The CV values for the different kits in the absence of MnCit werevery similar to those values reported by Rosenblum et al. (1997).The rhodamine kit in the absence of MnCit showed the highest CVvalues (56%-59%, Fig. 2; see Korch and Drabkin 1999). Additionof MnCit to the dRhodamine dye-terminator cycle-sequencing reactionsproduced electropherograms with the lowest CV values (18%). TheCVs of peak height for all primers with a specific kit were verysimilar (e.g., compare the dRhodamine results with the M13F andM13R primers in Fig. 2). In contrast, the BigDye sequencing resultsshowed the least amount of peak height variation in the absenceof MnCit, but addition of MnCit to these dye terminators onlyreduced the CV values from 32% to 24% (Fig. 2). Despite theseminor improvements in peak height uniformity, addition of ~0.4mM MnCit (in the presence of ~0.3 mM EDTA from solvent of kitcontrols; see below) caused a dramatic change in the color ofthe fluorescent gel image of the BigDye sequencing products. Thiscolor shift was due to reducing the relative strength of the Gsignals ~2.5-fold and increasing the relative strength of theC and T signals ~1.5-fold, making these dyes predominate (datanot shown).

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Figure 2 Increasing MnCit concentrations decrease the CVs of peak heights of different PE/ABI dye terminator sequencing kits. The data were obtained by sequencing with the kits, templates, and primers indicated. The curves of the CV values using the $-$ 21/pUC, M13F, M13R primers were determined by measuring the height of 100 nucleotide peaks as described in Methods, except the BigDye kit results with the $-$ 21/pUC primer are based on the fifty nucleotides 55-104. The dRhodamine and the BigDye sequencing results that contain the indicated amounts of EDTA were produced using the control $-$ 21/pUC primer and DNA template from the kits; whereas, the other results were obtained using our preparations of primers and pGEM3Zf(+) DNA that were dissolved in water.

The optimal MnCit concentration for each of the kits depended on the template and primer solvent. Using the $-$ 21/pUC primerand pGEM3Zf(+) template controls included in all three sequencingkits, peak height variability reached a minimum at ~0.6 mM MnCit(Fig. 2). In contrast when the primers and DNA were dissolvedin water, the optimal concentration of MnCit was ~0.3 mM MnCit.This discrepancy is due to the $-$ 21/pUC primer, and pGEM3Zf(+)template controls included in these sequencing kits are dissolvedin a Tris-EDTA buffer (TE), according to the manufacturer. However,this fact is not mentioned in the kit data sheets/instructions.Consequently, the final concentration of EDTA in the sequencingreaction would vary between 0.3 and 0.35 mM, depending on theamounts of each of the kit controls (primer and DNA) requiredfor sequencing with the different kits (see legend to Fig. 2 andMethods). This amount of EDTA raised the minimal concentrationof MnCit required to minimize peak height variability from ~0.3mM (Fig. 2, $black-triangle$ , $open circle$ , ) to ~0.6 mM (Fig. 2, $black-diamond$ , ). For consistentresults, we currently dissolve primers and DNA templates in eitherwater or 1-10 mM Tris-HCl (pH 8) and add 0.2-0.3 mM MnCit to thesequencingreactions.

MnCit Improves Sequencing Accuracy

Using pGEM3Zf(+) with either the M13F or $-$ 21/pUC primer, we tested the effect of adding MnCit on the accuracy of sequencedeterminations by comparing unedited base calls with the knownsequence of this plasmid. Optimal concentrations of MnCit significantlyincreased the accuracy of base calling by the computer algorithm.Figure 3 illustrates this effect on the number of miscalled basesfor the two newer dye-terminator sequencing kits. Earlier we notedthat with the rhodamine kit, MnCit significantly increased thetotal number of correctly called bases (on average, by 40 withinthe first 750 nucleotides) and extended the length of sequencewith equivalent base-calling accuracy by ~50-150 nucleotides (Korchand Drabkin 1999). The dRhodamine and BigDye sequencing kits producedmore accurate base calls than the rhodamine kit (cf. Figs. 3 and2 of Korch and Drabkin 1999). Addition of MnCit increased accuracywith the dRhodamine kit, but not with the BigDye kit. In reflectionof the MnCit effect on peak height uniformity, the dRhodaminekit with MnCit addition produced the most accurate sequence determinations(<11 miscalled bases between nucleotides 51 and 750), exceedingthe results seen with the BigDye kit (Fig. 3). Because of weaksignal strength in the first 50 nucleotides from the primer anddecreased resolution by the gel matrix above 500-600 bases, allthree kits showed elevated base-calling error rates in these regions.

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Figure 3 MnCit improves mean base-calling accuracy for the rhodamine and dRhodamine dye-terminator sequencing kits, but not for the BigDye kit. The template pGEM3Zf(+) was sequenced with either the M13F or the $-$ 21/pUC primer. The unedited base calls obtained using the different sequencing kits (without or with the addition of the optimal concentration of MnCit) were aligned with the known sequence of pGEM3Zf(+). The percent miscalled bases was determined for each 50-nucleotide increment, as measured from the 3' end of the sequencing primer. In the increment 1-50, the error rate calculations do not include bases not detected, but only those incorrectly called. The mean dRhodamine values are based on 6 and 10 sequences in the absence ( $black-triangle$ ) and presence ( $triangle$ ) of MnCit, respectively. The mean BigDye values are based on four and six sequences in the absence (

) and presence (

) of MnCit, respectively. Error bars are not shown for clarity.

Generally, the 5'-AG-3' dinucleotides are the most problematic for accurate base calling because of the so-called "suppression"of Gs that follow As. Additions of optimal amounts of MnCit significantlyreduced G suppression for both the rhodamine (shown earlier) anddRhodamine results. In many cases, the G peak following an A wasas tall or taller than the A peak (see nucleotides 300-310 inFig. 1). With the templates we used, no other systematic base-callingerrors wereobserved.

MnCit Improves Detection of Genetic Heterozygosities

The discovery that addition of MnCit to the rhodamine- and dRhodamine-sequencing reactions greatly reduced peak height variationssuggested that MnCit-modified dye-terminator sequencing reactionscould be used in the analysis of heterozygosity in PCR-amplifiedproducts. On comparing the sequencing results in the absence andpresence of MnCit for an ~1:1 mixture of two plasmids differingat specific nucleotide positions, it is clear that MnCit makesit easier to visually detect the presence of two bases at theindicated positions of the mutations (Fig. 4). For example, inthe mixed template sequence ("heterozygous" condition) in Figure4A, the site of the mutation appears as a suppressed G in theabsence of MnCit (compare with the height of the suppressed Gpeaks surrounding the mutation). Addition of MnCit produces peaksof more uniform height except at this site, where the peaks aredistinguishable and about one-half their average height. By visualexamination of the Figure 4A electropherograms, the site of mixedbases in the presence of MnCit can be seen as a depression inthe uniform peak profile, making it easier to identify those regionsof potential heterozygosity that need to be confirmed by sequencingof the complementary DNA strand. Also, base calling is improvedby MnCit addition as is evident upstream of the mutation in Figure4A, where there are two Gs that in the absence of MnCit appearas one because of G suppression.

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Figure 4 MnCit addition improves detection of heterozygous mutations. Compared are DNA sequence electropherograms produced by sequencing different pairs of plasmids with dRhodamine reagents in the absence ( $-$ ) and the presence (+) of 0.2 mM (A) or 0.3 mM (B,C) MnCit. The templates were approximately equimolar mixtures of two plasmids containing segments of DNA that differed by single nucleotides. The arrows and letters indicate the sites of a suppressed G (G sup); mixed peaks are attributable to the DNA sequences corresponding to heterozygous mutations (e.g., G + A), with the upper letter being the taller peak; and a T peak (T) that is strong in the template with the sequence 5'-GATC-3', but not in the template with the sequence 5'-AATC-3' (data not shown).

However, MnCit addition does not even out all peak heights to produce this depression effect. Instead, MnCit addition increasedthe strength of some weak peaks so that the heterozygous siteis more clearly evident as a peak of mixed bases (Fig. 4B,C).Moreover, higher than optimal MnCit concentrations produce threesequence profile anomalies with the rhodamine- and dRhodamine-sequencingkits. Unlike most G peaks, the strength of G peaks in the sequence5'-CTG-3' increased disproportionately with increasing concentrationsof Mn²⁺. This effect was stronger if the G preceded pyrimidines ratherthan purines (data not shown). In a complement of this sequence(i.e., 5'-CCAG-3'), elevated levels of Mn²⁺ caused a slight misincorporation of G dye terminator insteadof A dye terminator, giving rise to an A peak with an underlyingG peak in these sequences (data not shown). In addition, althoughoptimal amounts of MnCit produced very uniform peak heights withthe dRhodamine dye-terminator kits, Ts in the sequence 5'-GATC-3'were clearly stronger than the surrounding signals. This effect,evident in Figure 4C because one of the two variant templateshas the sequence 5'-GATC-3', produced a strong T peak in the mixedtemplates. Therefore, to avoid mistaking a heterozygosity in thesequence with one of these anomalies and to use them to flag potentialsites of mixed bases, the optimal MnCit concentration should bedetermined for nonmutant DNA template and primer combinations,with both dissolved inwater.

	DISCUSSION

Top Abstract Introduction RESULTS DISCUSSION METHODS References

Tabor and Richardson (1989, 1995) compared the ability of three DNA polymerases (from phage T7, Escherichia coli, and T. aquaticus)to discriminate against ddNTPs in the presence of either 5 mMMg²⁺ or 2 mM Mn²⁺. Substitution of manganese for magnesium reduced the discriminationagainst ddNTPs by 4- to 100-fold. As a result, manganese withtrisodium isocitrate has been reported to improve peak heightuniformity using T7 and E. coli DNA polymerases (Fuller 1989;Tabor and Richardson 1989, 1990) and the thermostable DNA polymerasesTaq (Brandis et al. 1996) and Tub (Rao and Saunders 1992). Inthe case of the Taq and Tub polymerases, variability in peak heightsis much greater than that seen with wild-type T7 DNA polymeraseand the mutant Sequenase. Tabor and Richardson (1995) reportedthat substitution of manganese for magnesium had no significanteffect on ddNTP incorporation by the F667Y mutant Taq DNA polymerase(i.e., the enzyme in the PE/ABI kits). In contrast, Brandis etal. (1996) reported that KlenTaq (a genetically engineered formof Taq DNA polymerase lacking the 5' to 3' exonuclease domain)was strongly inhibited by manganese in the absence of magnesiumand isocitrate or citrate. They did not report testing the combinedeffect of manganese in the presence of magnesium. Although manganesereduced peak height variability with KlenTaq, they concluded thatthe improvements were insufficient to warrant its routine use,because of the severe inhibition of enzymaticactivity.

Recently, we demonstrated that the uniformity of sequencing peak heights could by improved by addition of MnCit to a DNA cycle-sequencingreaction based on rhodamine dye terminators with a F667Y mutantTaq DNA polymerase (Korch and Drabkin 1999). Here, we comparethe improvements produced by MnCit with the rhodamine-based, dRhodamine,and BigDye dye-terminator sequencing kits in a reaction mixture.With these kits, the most dramatic effect of Mn²⁺ addition is to reduce the discrimination by this DNA polymeraseagainst all dye terminators, especially increasing the incorporationof dye-labeled ddGTPs following incorporation of an unlabeleddAMP in the sequence (see Fig. 1). Rao and Saunders (1992) noteda related phenomenon when they determined with Tub DNA polymerasethat the least amount of manganese was needed to significantlyincrease incorporation of ddGMPs as opposed to the incorporationof other dideoxynucleotides (0.2 mM vs. 0.4-0.6 mM).

In the absence of metal chelators such as EDTA, the optimal Mn²⁺ concentration is ~0.3 mM. Addition of equimolar amounts of thetrisodium salts of either citrate or isocitrate further improvesthe uniformity. To obtain the most consistent MnCit optimization,it is critical not to dissolve the DNAs and primers in bufferscontaining metal chelators, such as EDTA. Normally, differencesin DNA concentration between samples are compensated by adjustingthe sample volume to obtain optimal signal strengths in DNA sequencingreactions. As a consequence, the amount of EDTA added to the reactionwould vary and therefore, different concentrations of MnCit wouldbe required to minimize peak height variability. To avoid thiscomplication, the DNAs and primers should be dissolved in wateror a weak buffer (1-10 mM Tris-HCl, pH 8). To compensate for theinhibitory effect of MnCit and to avoid producing artifacts resemblingheterozygous sequences, it may be necessary to determine the optimalconcentrations of MnCit, DNA, and primers for differentapplications.

Although the newer dRhodamine- and BigDye-based sequencing methodologies produce less variation in peak heights than the rhodamine-basedmethod (Zakeri et al. 1998; this paper), they cannot be used onthe PE/ABI 373A sequencer without a costly upgrade of the filterwheel, which because of spectral incompatibilities cannot be usedwith the dyes on genotyping primers. As we pointed out earlier(Korch and Drabkin 1999), addition of MnCit to the rhodamine-baseddye-terminator sequencing reactions can therefore eliminate theneed for this upgrade and retain the versatility of this sequencer.Using this instrument with 48-cm [well-to-read (WTR)] 5% LongRanger gels and the rhodamine kit with MnCit addition, we foundthe first N in the sequence usually appeared after 650 nucleotidesfrom theprimer.

Furthermore and significantly, the dRhodamine-based dye-terminator sequencing chemistry with the addition of MnCit produceselectropherograms with the most uniform peak height, even moreuniform than those produced by the energy-transfer dyes (BigDyes),resulting in the most accurate sequence determinations. In fact,the dRhodamine kit with 0.3 mM MnCit yielded a CV of 18%. In comparison,Rosenblum et al. (1997) obtained a CV of 26% for sequencing thesame DNA with dye-labeled primers. Also, we calculated a CV of35% from dye-primer data from McDonald et al. (1995). Consequently,the MnCit improvement of the dRhodamine sequencing kit producesthe most uniform peak heights, making it ideal for the identificationof heterozygous mutations in mixedtemplates.

	METHODS

Top Abstract Introduction RESULTS DISCUSSION METHODS References

Template and Primer Preparation

The DNA template used for most of these studies, pGEM3Zf(+) (Promega Corporation, Madison, WI), was either used as providedin the sequencing kits by PE/ABI (dissolved in TE buffer: 10 mMTris-HCl at pH 8, 1 mM EDTA) or prepared as described earlier(Korch and Drabkin 1999) and dissolved in water. The sequencingprimers, listed below, were synthesized by GIBCO/BRL Life Technologies(Gaithersburg, MD) and dissolved in water, with the exceptionof the $-$ 21/pUC primer, which has the same sequence as the M13forward (M13F) primer, but was supplied by PE/ABI in the sequencingkits and is dissolved in a TE buffer. The sequences of the primerstested in this study are (5' $right-arrow$ 3'): $-$ 21/pUC and M13F (TGTAAAACGACGGCCAGT);T7 (TAATACGACTCACTATAGGG); M13R (TCACACAGGAAACAGCTATGAC); M13RGC+ (GCTATGACCATGATTACGCC); M13 GC $-$ (GGAAACAGCTATGACCATGATTA);SP6 (GCTATTTAGGTGACACTATAGAA); SP6 GC+ (CCAAGCTATTTAGGTGACAC);and T3 (ATTAACCCTCACTAAAGGGA). The T3 primer was tested by sequencingplasmids based on pBlueScript SK( $-$ ) from Stratagene (La Jolla,CA).

DNA Sequencing Protocol

DNA template (400 ng) was mixed with sequencing primer (0.8-50 pmoles) and 3 µl of AmpliTaq DNA polymerase FS mixture in atotal volume of 10 µl. Dye-terminator cycle sequencing was performedas recommended by the manufacturer and described earlier (Korchand Drabkin 1999). We tested the dye-terminator sequencing kitsfrom PE/ABI using ddNTPs labeled with (1) rhodamine-based dyes(rhodamine kit; PE/ABI Prism Dye-Terminator Cycle-Sequencing ReadyReaction kit with AmpliTaq DNA polymerase FS); (2) dichloro-rhodamine-baseddyes (dRhodamine kit; PE/ABI Prism dRhodamine Terminator Cycle-SequencingReady Reaction Kit with AmpliTaq DNA polymerase FS); and (3) energy-transferdichlororhodamine-based dyes (BigDye kit; PE/ABI Prism BigDyeTerminator Cycle-Sequencing Ready Reaction Kit with AmpliTaq DNApolymerase FS). Reactions using the dRhodamine and BigDye terminatorscontained 600 and 200 ng of pGEM3Zf(+) DNA,respectively.

MnCit solutions (2-10 mM) were made by mixing equal volumes of a 100 mM solution of manganese acetate tetrahydrate, manganesechloride tetrahydrate, or manganese sulfate monohydrate with a100 mM solution of either trisodium citric acid dihydrate or trisodiumDL-isocitrate monohydrate and diluting to make mixed stock solutionswith final concentrations of 2-10 mM of each component and storedat $-$ 20°C. An aliquot (0.5-4 µl per 10-µl final reaction volume)of one of the mixed stock solutions was added to the sequencingreaction mixtures to produce the desired finalconcentration.

Excess dye-labeled terminators and buffers were removed by ethanol precipitation at room temperature. To each 10- or 20-µlreaction volume, 50 µl of 0.3 mM sodium acetate (pH ~ 5, roomtemperature) was added and the mixture was transferred to a microcentrifugetube containing 125 µl of 100% ethanol (room temperature) andmixed by vortexing. The mixtures were stored at room temperaturefor 20 min and centrifuged in a microcentrifuge at maximum speedat room temperature. The supernatant was slowly decanted to removethe supernatant and the last drop was blotted onto paper towels.The pellets were rinsed with 1 ml of 70% ethanol (vol/vol in water),vortexed, and centrifuged as above for 10 min. Subsequently, thesupernatant was decanted very slowly so the film of 70% ethanolformed as few droplets as possible on the side of the centrifugetube. The final droplets were removed by tapping the tubes upsidedown on paper towels. For the Big Dye reactions, an additionalrinse with 70% ethanol was required. Less than 5 µl of rinsingsolution should be left in the tube. The samples were dried ina Speed-Vac (Savant Instruments, Holbrook, NY). The pellets wereresuspended by vortexing with 3 or 4 µl of loading buffer (5:1mixture of 100% freshly deionized formamide/2.5% blue dextranin 25 mM EDTA at pH 8). Samples were heated for 2-3 min at ~95°C,cooled on ice, and 1.75 µl was applied to a 34-cm (WTR), 0.2-mm-thickgel of the PE/ABI 377. Alternatively, a 3-µl sample was appliedto a 48-cm WTR, 0.3-mm thick gel of an PE/ABI 373A. The PE/ABI377 (34-cm) gels were made with 1× TBE (89 mM Tris, 89 mM borate,2 mM EDTA), 6 M urea with either 4.2% polyacrylamide/bis-acrylamide(19:1) or using 5.0% Long Ranger polyacrylamide matrix (FMC Bioproducts,Rockland, ME). The PE/ABI 373A (48-cm) gels were made of 8.3 Murea, 1× TBE, and either 4.75% polyacrylamide/bisacrylamide (19:1)or 5% Long Rangermatrix.

Analysis of Sequence Data

Data were collected on the different instruments with the PE/ABI Prism 373 DNA-Sequencing System Data Collection (v. 1.2.1)and the PE/ABI Prism 377 DNA Sequencer Data Collection (v. 1.1).Sequence analysis was done with the PE/ABI Prism DNA-SequencingSoftware (v. 2.1.1). Peak height variability was determined eitherby visual inspection of the electropherogram or by measuring theheight of 50 or 100 individual peaks on the printed electropherograms.For the $-$ 21/pUC, T7, and M13F primers, these peaks correspondedto nucleotides 55 (base 1 of the XbaI site) through 104 or 154nucleotides from the 3' end of the $-$ 21/pUC or M13F primer on theplasmid pGEM3Zf(+) (GenBank accession no. X65306). For theM13R primer, the peaks corresponded to bases 135-234 from the3' end of the primer on the same template DNA. Coefficients ofvariations (CVs = 100% ·[S.D./mean]) of the peak heights weredetermined for all bases in these regions as well as for eachof the four bases. Base-calling accuracy was determined by comparingthe sequence called by the PE/ABI algorithm to the known sequenceof pGEM3Zf(+) as described earlier (Korch and Drabkin 1999). Therelative incorporation of dye-labeled terminators was estimatedby summation of the average strength of peak signals for the fourbases. These estimates of "activity" are subject to inaccuraciesin loading small samplevolumes.

Mixing of plasmid DNAs containing variants of different genes (obtained from R. Calvo and H. Drabkin) were performed to testfor the effect of MnCit on the detection of heterozygous mutations.The DNA concentrations were quantified by (1) visual estimationsof band intensities after electrophoresis on agarose gels containingethidium bromide and (2) sequencing the individual plasmids andusing the sum of the average strength of peak signals for thefour bases. Sample volumes containing equivalent amounts of DNAwere mixed and sequenced with the T7 primer together in eitherthe absence or presence ofMnCit.

	ACKNOWLEDGMENTS

We are indebted to Ms. Christina Desseva and Ms. Efang Li for their excellent technical assistance and to Dr. Roser Calvofor the use of plasmids bearing gene variants. This work was supportedby the National Institutes of Health (NIH)-National Center forHuman Genome Research grant 5R01 HG00358 to H.D. and by the NIH-NationalCancer Institute grant CA46934 to the UCCC for support of theUCCC DNA Sequencing & AnalysisCore.

The publication costs of this article were defrayed in part by payment of page charges. This article must therefore be herebymarked "advertisement" in accordance with 18 USC section 1734solely to indicate thisfact.

	FOOTNOTES

³ Correspondingauthor.

E-MAIL christopher.korch{at}uchsc.edu; FAX (303) 315-8825.

REFERENCES

Top
Abstract
Introduction
RESULTS
DISCUSSION
METHODS
References

Brandis, J.W., S.G. Edwards, and K.A. Johnson. 1996. Slow rate of phosphodiester bond formation accounts for the strong bias that Taq DNA polymerase shows against 2',3'-dideoxynucleotide terminators. Biochemistry 35: 2189-2200[CrossRef][Medline].
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Received February 18, 1999; accepted in revised form May 3, 1999.

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METHODS Improved DNA Sequencing Accuracy and Detection of Heterozygous Alleles Using Manganese Citrate and Different Fluorescent Dye Terminators

METHODS
Improved DNA Sequencing Accuracy and Detection of Heterozygous Alleles Using Manganese Citrate and Different Fluorescent Dye Terminators