WO1996023807A1 - Novel chain terminators, the use thereof for nucleic acid sequencing and synthesis and a method of their preparation - Google Patents

Novel chain terminators, the use thereof for nucleic acid sequencing and synthesis and a method of their preparation Download PDF

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Publication number
WO1996023807A1
WO1996023807A1 PCT/SE1996/000096 SE9600096W WO9623807A1 WO 1996023807 A1 WO1996023807 A1 WO 1996023807A1 SE 9600096 W SE9600096 W SE 9600096W WO 9623807 A1 WO9623807 A1 WO 9623807A1
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group
compound
formula
nucleic acid
compounds
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PCT/SE1996/000096
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French (fr)
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Marek Kwiatkowski
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Marek Kwiatkowski
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Priority to US08/875,243 priority Critical patent/US6255475B1/en
Priority to JP8523466A priority patent/JPH10513178A/en
Priority to EP96902039A priority patent/EP0808320B1/en
Priority to DE69627314T priority patent/DE69627314T2/en
Publication of WO1996023807A1 publication Critical patent/WO1996023807A1/en

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    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07HSUGARS; DERIVATIVES THEREOF; NUCLEOSIDES; NUCLEOTIDES; NUCLEIC ACIDS
    • C07H19/00Compounds containing a hetero ring sharing one ring hetero atom with a saccharide radical; Nucleosides; Mononucleotides; Anhydro-derivatives thereof
    • C07H19/02Compounds containing a hetero ring sharing one ring hetero atom with a saccharide radical; Nucleosides; Mononucleotides; Anhydro-derivatives thereof sharing nitrogen
    • C07H19/04Heterocyclic radicals containing only nitrogen atoms as ring hetero atom
    • C07H19/16Purine radicals
    • C07H19/20Purine radicals with the saccharide radical esterified by phosphoric or polyphosphoric acids
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07HSUGARS; DERIVATIVES THEREOF; NUCLEOSIDES; NUCLEOTIDES; NUCLEIC ACIDS
    • C07H19/00Compounds containing a hetero ring sharing one ring hetero atom with a saccharide radical; Nucleosides; Mononucleotides; Anhydro-derivatives thereof
    • C07H19/02Compounds containing a hetero ring sharing one ring hetero atom with a saccharide radical; Nucleosides; Mononucleotides; Anhydro-derivatives thereof sharing nitrogen
    • C07H19/04Heterocyclic radicals containing only nitrogen atoms as ring hetero atom
    • C07H19/06Pyrimidine radicals
    • C07H19/10Pyrimidine radicals with the saccharide radical esterified by phosphoric or polyphosphoric acids
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
    • C12Q1/00Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
    • C12Q1/68Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving nucleic acids
    • C12Q1/6869Methods for sequencing

Definitions

  • the present invention relates to novel nucleic acid chain extension terminators, their use in nucleic acid sequencing and synthesis, respectively, as well as a method for preparing such compounds.
  • primers to which deoxynucleotides and dideoxynucleotides are added are dye- labelled, or the added dideoxynucleotides are
  • dye labelled deoxynucleotides can be used in conjunction with unlabeled dideoxynucleotides. This chain termination method is based upon the ability of an enzyme to add specific nucleotides onto the 3' hydroxyl end of a primer annealed to a
  • the extension products are then separated electrophoretically on a polyacrylamide gel and detected by an optical system utilizing laser excitation.
  • the SBH methods are problematic in several respects.
  • the hybridization is dependent upon the sequence composition of the duplex of the oligonucleotide and the polynucleotide of interest, so that GC-rich regions are more stable than AT-rich regions.
  • false positives and false negatives during hybridization detection are frequently present and complicate sequence determination.
  • sequence of the duplex of the oligonucleotide and the polynucleotide of interest so that GC-rich regions are more stable than AT-rich regions.
  • polynucleotide is not determined directly, but is inferred from the sequence of the known probe, which increases the possibility for error.
  • Hyman E.D., Anal. Biochem., 174:423 (1988) discloses the addition of a nucleotide to a an immobilised DNA template/primer complex in the presence of a polymerase and determination of polymerisation reaction by detecting the pyrophosphate liberated as a result of the polymerisation.
  • Jett et al. J. Biomol. Struct. Dyn., I, p. 301, 1989 discloses a method wherein a single stranded DNA or RNA molecule of labelled nucleotides, complementary to the sequence to be determined, is suspended in a moving flow stream. Individual bases are then cleaved sequentially from the end of the suspended sequence and determined by a detector passed by the flow stream.
  • EP-A-223 618 discloses the use of an immobilised DNA template, primer and polymerase exposed to a flow
  • a downstream detection system determines whether deoxynucleotide is incorporated into the copy or not by detecting the difference in deoxynucleotide concentrations entering and leaving the flow cell containing the complex of DNA template and polymerase.
  • WO 90/13666 proposes a method directly measuring the growth of the template copy rather than determining it indirectly from compositions in the flow medium. Only one of the four nucleotides is present at a time, and the polymerisation events reflecting the incorporation of a nucleotide or not are detected by spectroscopic means (evanescent wave spectroscopy, fluorescence detection, absorption spectroscopy) or by the individual nucleotides being labelled.
  • spectroscopic means evanescent wave spectroscopy, fluorescence detection, absorption spectroscopy
  • One object of the present invention is to provide novel nucleotide derivatives which may be used as chain terminators and which by deprotection may readily be converted into nucleotides or nucleotide analogues that may be further extended.
  • Another object of the present invention is to provide a method for nucleotide sequence determination using the novel chain terminators.
  • nucleotide or nucleotide analogue having its 3'-hydroxyl group protected by an acetal or thioacetal structure designed in such a way that the 3'-hydroxyl can be
  • dilute acid such as hydrochloric acid at pH 2, for example.
  • the present invention therefore provides a compound of the general formula I:
  • B is a nucleobase
  • X and Z independently are oxygen or sulphur
  • Y is hydrogen, hydroxy or protected hydroxy, such as methoxy, ethoxy or allyloxy,
  • R 1 is hydrocarbyl, which optionally is substituted with a functional group
  • R 2 is hydrogen or hydrocarbyl, which optionally is substituted with a functional group
  • A is an electron withdrawing or electron donating group capable of moderating the acetal stability of the compound I via L 1 , L 1 and 1-2 are hydrocarbon linkers, which may be the same or different, L 2 , when present, being either (i) connected to L 1 via the group A, or (ii) directly
  • F is a dye label
  • Q is a coupling group for F
  • 1, m and n independently are O or 1, with the proviso that 1 is 1 when m is 1, and 1 is 1 and m is 1 when n is 1.
  • nucleobase B may be natural or synthetic. Natural nucleobases include common
  • nucleobases such as adenine, guanine, cytosine, thymine and uracil, as well as less common nucleobases, such as xanthine, hypoxanthine or 2-aminopurine.
  • nucleobases B are analogues to the natural nucleobases and capable of interacting with other nucleobases in a
  • the hydrocarbyl groups represented by R 1 and R 2 include a wide variety, including straight and branched chain alkyl, alkenyl, aryl, aralkyl and cycloalkyl, preferably containing up to 10 carbon atoms.
  • Preferred hydrocarbyl groups are primary, secondary or tertiary alkyl, alkenyl or alkynyl groups, especially lower alkyl groups, such as methyl and ethyl.
  • the optional functional group substituents on R 1 and R 2 are capable of moderating the lability of the 3' acetal group through an inductive effect. Exemplary of such functional groups are tert.
  • Detectable moiety, or label F can be chosen from a vast number of such moieties known to those skilled in the art. Exemplary such moities are radioactively labeled functions, luminescent, electroluminescent or fluorescent labels, and labels that absorb characteristic visible or infrared light. Preferably, F is a fluorescent label.
  • a large number of such coupling groups capable of reacting with and binding label F via a reactive function thereon are known to those skilled in the art. Examples of reactive groups are amino, thio, and carboxyl.
  • the group Q is derived completely from the reactive function on the uncoupled F.
  • the coupling reaction is a substitution reaction
  • the group reacting with F being, for example, a halogen (fluoride, chloride, bromide or iodide)
  • the group Q will be represented by the reactive function present on label F.
  • Electron withdrawing or donating group A is
  • the group A may represent a part of the chain L 1 -A-L 2 .
  • Representative groups A in that case are amido, sulfoxy, sulfone, carbalkoxy (ester), ether, thioether and amino groups.
  • A may be a side substituent for the L 1 -L 2 chain, representative groups then being, for example, cyano, nitro and halogen (halogen including fluoride, chloride, bromide and iodide).
  • linker L 1 will donate structure stretching from the acetal carbon to the place of the substitution
  • linker L 2 will donate structure stretching from this substitution to the group A. It is to be emphasized that the specific electron withdrawing and electron donating groups
  • hydrocarbon linker L 1 will be selected with regard to the function A, inductive effects being highly depending on distance. While a straight aliphatic (saturated or unsaturated) hydrocarbon chain is preferred, branched or cyclic hydrocarbons may be contemplated. Preferably, linker L 1 has up to 10 carbon atoms, more preferably up to 6 carbon atoms.
  • hydrocarbon linker L2 The function of hydrocarbon linker L2 is to provide, together with linker L 1 , A and coupling group Q, for a sufficiently long distance between the label moiety F and the rest of the compound of Formula I. This is required by spatial preferences of the enzymes (polymerases) for which the compound of Formula I acts as substrate or by the necessity of avoiding interaction between the label and nucleobase B. It is readily understood that the structure of linker L 2 highly depends on the particular enzyme, label F and possibly also nucleobase B that are used. A suitable length and structure of linker L 2 will therefore be selected by the skilled person for each particular situation. Similarly as for linker L 1 , a preferred
  • linker L2 is a straight aliphatic (saturated or unsaturated) hydrocarbon chain, although branched or cyclic hydrocarbons may be contemplated.
  • linker L 2 has up to 10 carbon atoms, more preferably up to 6 carbon atoms.
  • linker L2 may, of course, also be omitted.
  • the compounds of Formula I can be deprotected to exhibit a free 3'-hydroxy group in a relatively short time under acidic conditions, e.g. with hydrochloric acid at about pH 2. It is understood that by proper selection of the groups R 1 , R 2 , A, L 1 and L 2 with regard to each other, the deprotection time may be adjusted to a desired range. Under the mentioned acidic conditions, the most preferred compounds of Formula I will be deprotected within, say, 0.01 to 15 minutes.
  • Another aspect of the invention therefore provides a method for determining the sequence of a nucleic acid, which method comprises providing a single-stranded
  • nucleic acid template comprising the nucleic acid to be determined, and at least partially synthesizing a complementary nucleic acid molecule in a stepwise serial manner by the addition of nucleotides in which the identity of each nucleotide incorporated into the complementary nucleic acid molecule is determined subsequent to its incorporation, wherein said nucleotides are compounds of Formula I as defined above, and wherein the 3'-blocking group is removed from the nucleotide after its incorporation to permit further extension of the nucleic acid molecule.
  • a method for determining the sequence of a nucleic acid comprises the following steps : (i) providing a single-stranded template comprising the nucleic acid to be sequenced,
  • step (iii) may be added in sequence, in which case the four different compounds I may carry the same label F. Alternatively, the different compounds I have different labels F and are added at the same time.
  • the template/primer complex is bound to a solid-phase support, such as a sequencing chip, for example.
  • a solid-phase support such as a sequencing chip
  • the template may be attached to the solid support via a binding linker, which, for instance, is ligated to the 5'-end of the template or incorporated in one of the ends of the template by polymerase chain reaction (PCR).
  • PCR polymerase chain reaction
  • the binding linker may then be attached to the solid support by use of a streptavidin coupling system.
  • the primer may be attached to the solid support.
  • the compounds of Formula I may, of course, also conveniently be used in so-called mini-sequencing (see e.g. Syvanen A-C et al., Genomics 8:684-692 (1990).
  • the compounds of Formula I may also be used in the synthesis of nucleotide chains, and another aspect of the invention relates to such use.
  • the compounds of Formula I may also be used in the synthesis of nucleotide chains, and another aspect of the invention relates to such use.
  • oligonucleotides and polynucleotides may be prepared by successively coupling compounds of Formula I to each other in any desired base order with intervening deblocking and using a non-template dependent polymerase, such as a terminal transferase.
  • a non-template dependent polymerase such as a terminal transferase.
  • the groups L 2 , Q and F in Formula I may, of course, be omitted.
  • the compounds of Formula I may be prepared by methods known per se. In a further aspect, however, the invention provides a particular method for the preparation of a subgroup of compounds of Formula I by direct 3'-OH
  • B, X, Z, R 1 , R 2 , p and q are as defined above, and optionally coupling a dye label F to the terminal amino group.
  • Fig. 1 is a reaction scheme for the enolether
  • Fig. 2 is a reaction scheme for the preparation of 3'-acetal-modified thymidine described in Example 2 below. Prepared final compounds corresponding to various values of integer "n" in the respective structural formula are identified by numbers indicated within brackets after the n-values listed under the formula.
  • Fig. 3 is a graph showing thymidine 3'-acetal
  • Fig. 4 is a reaction scheme for the one-pot synthesis of 3'-acetal protected deoxynucleotide triphosphates described in Example 4 below.
  • Intermediate and final products corresponding to various values of integer "n" in the respective structural formulae are identified by numbers indicated within brackets after the n-values listed under the respective formulae.
  • ketoacids were used:
  • the material homogeneous by TLC (developed in 1-butanol -ammonium hydroxide 8:2), was combined, evaporated, and coevaporated with toluene, to give the NMR pure product (compounds 9-12 in Fig. 2) in high yield (72 to 85%) .
  • the pure material was stored as a stock solution in methanol after addition of three drops of ammonia.
  • triethylammonium salt This material was evaporated on a Rotavapor, coevaporated with dry acetonitrile (3 ⁇ 2 ml), and dissolved in molecular sieve-dried trimethylphosphate (0.5 ml).
  • the appropriate enolether (compounds 5-8 in Fig. 1) (0.2 ml) and trifluoroacetic acid (10 eq as a 10% solution in dry dioxane) were added.
  • the homogeneous mixture was incubated at 20°C for 60 min, neutralized by the addition of triethylamine (100 ml), and precipitated from a 1:1 mixture of petroleum ether and diethyl ether.
  • Thymidine triphosphate reacts to form, besides the desired 3' -modified derivative, also another product with even shorter retention time but that also hydrolyses to the starting triphosphate during acid treatment. It is assumed that this product is the bis-3'-O, 4-O-acetal-derivative of thymidine triphosphate. This type of side products was not present in reactions that used other nucleotide triphosphates. It should also be stressed that very little products of depurination were formed in reactions in which pppdG and pppdA were used. This can be explained by the mild acid applied as a catalyst, the large excess of enolether used in the reaction, and the fact that the bases existed in an unprotected (more acid resistant) form.
  • oligonucleotides were prepared, having sequences corresponding to the M13 sequencing primer, and designed to incorporate to their 3'-ends T, G, A or C base
  • each of the labelled primers was subjected to the single step extension conditions.
  • These reaction mixtures (20 ml) were composed of the respective primer (0.1 pmol), M13 template (1 pmol), and 3'-modified thymidine triphosphate (compound 16 in Fig. 4) in a buffer system pH 7.5 containing Tris/HCl (40 mM), MnCl 2 (4 mM), dithiothreitol (DTT) (11 mM), sodium isocitrate (29 mM) and sodium chloride (23 mM).
  • the sequencing reactions consisted of the following components: M13 mp 18 ss-DNA template (1 pmol), 5'-fluorescein labelled universal primer (1 pmol, Pharmacia Biotech AB), Ampli Taq DNA polymerase (4U) and T-termination mixture in cycle sequencing buffer (Tris-HCl pH 8.9, 80 mM, ammonium sulfate 20 mM, magnesium chloride 5 mM).
  • cycle sequencing buffer Tris-HCl pH 8.9, 80 mM, ammonium sulfate 20 mM, magnesium chloride 5 mM.
  • compound 16 in Fig. 4 in different proportions with TTP, was used as a chain terminator.
  • an equal volume of formamide was added and the mixture was heated for 2 min at 90°C, cooled on ice and loaded onto 6% acrylamide urea gel. Separation and analysis of products were performed on an A.L.F. DNA-sequencer (Pharmacia)

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Abstract

The invention relates to compounds of general structure (I) or salts thereof, wherein B is a nucleobase, X and Z independently are oxygen or sulphur, Y is hydrogen or hydroxy, which optionally may be protected, R1 is hydrocarbyl, which optionally is substituted with a functional group, R2 is hydrogen or hydrocarbyl, which optionally is substituted with a functional group, A is an electron withdrawing or electron donating group capable of moderating the acetal stability of compound (I), L1 and L2 are hydrocarbon linkers, which may be the same or different, L2, when present, being either (i) connected to L1 via the group A, or (ii) directly connected to L1, the group A then being connected to one of linkers L1 and L2, F is a dye label, Q is a coupling group for F, and 1, m and n independently are 0 or 1, with the proviso that 1 is 1 when m is 1, and 1 is 1 and m is 1 when n is 1. The compounds of formula (I) are useful as deactivatable chain extension terminators. The invention also relates to the use of the compounds (I) in nucleic acid synthesis and nucleic acid sequencing as well as to a method of preparing compounds of Formula (I).

Description

NOVEL CHAIN TERMINATORS, THE USE THEREOF FOR NUCLEIC ACID SEQUENCING AND SYNTHESIS AND A METHOD OF THEIR PREPARATION
The present invention relates to novel nucleic acid chain extension terminators, their use in nucleic acid sequencing and synthesis, respectively, as well as a method for preparing such compounds.
Today, there are two predominant methods for DNA sequence determination: the chemical degradation method (Maxam and Gilbert, Proc. Natl. Acad. Sci. 74:560-564
(1977), and the dideoxy chain termination method (Sanger et al., Proc. Natl. Acad. Sci. 74:5463-5467 (1977)). Most automated sequencers are based on the chain termination method utilizing fluorescent detection of product
formation. In these systems either primers to which deoxynucleotides and dideoxynucleotides are added are dye- labelled, or the added dideoxynucleotides are
fluorescently labelled. As an alternative, dye labelled deoxynucleotides can be used in conjunction with unlabeled dideoxynucleotides. This chain termination method is based upon the ability of an enzyme to add specific nucleotides onto the 3' hydroxyl end of a primer annealed to a
template. The base pairing property of nucleic acids determines the specificity of nucleotide addition. The extension products are then separated electrophoretically on a polyacrylamide gel and detected by an optical system utilizing laser excitation.
Although both the chemical degradation method and the dideoxy chain termination method are in widespread use, there are many associated disadvantages. For example, the methods require gel-electrophoretic separation. Typically, only 400-800 base pairs can be sequenced from a single clone. As a result, the systems are both time- and labor- intensive. Methods avoiding gel separation have been developed in attempts to increase the sequencing
throughput.
Sequencing by hybridization (SBH) methods have been proposed by Crkvenjakov (Drmanac et al., Genomics 4:114 (1989); Strezoska et al., (Proc. Natl. Acad. Sci. USA
88:10089 (1991)), Bains and Smith (Bains and Smith, J. Theoretical Biol. 135:303 (1988)) and in US-A-5, 202, 231. This type of system utilizes the information obtained from multiple hybridizations of the polynucleotide of interest, using short oligonucleotides to determine the nucleic acid sequence. These methods potentially can increase the sequence throughput beacuse multiple hybridization
reactions are performed simultaneously. To reconstruct the sequence, however, an extensive computer search algorithm is required to determine the most likely order of all fragments obtained from the multiple hybridizations.
The SBH methods are problematic in several respects. For example, the hybridization is dependent upon the sequence composition of the duplex of the oligonucleotide and the polynucleotide of interest, so that GC-rich regions are more stable than AT-rich regions. As a result, false positives and false negatives during hybridization detection are frequently present and complicate sequence determination. Furthermore, the sequence of the
polynucleotide is not determined directly, but is inferred from the sequence of the known probe, which increases the possibility for error.
Methods have also been proposed which detect the addition or removal of single molecules from a DNA strand.
For example, Hyman E.D., Anal. Biochem., 174:423 (1988) discloses the addition of a nucleotide to a an immobilised DNA template/primer complex in the presence of a polymerase and determination of polymerisation reaction by detecting the pyrophosphate liberated as a result of the polymerisation.
Jett et al., J. Biomol. Struct. Dyn., I, p. 301, 1989 discloses a method wherein a single stranded DNA or RNA molecule of labelled nucleotides, complementary to the sequence to be determined, is suspended in a moving flow stream. Individual bases are then cleaved sequentially from the end of the suspended sequence and determined by a detector passed by the flow stream. EP-A-223 618 discloses the use of an immobilised DNA template, primer and polymerase exposed to a flow
containing only one species of deoxynucleotide at a time. A downstream detection system then determines whether deoxynucleotide is incorporated into the copy or not by detecting the difference in deoxynucleotide concentrations entering and leaving the flow cell containing the complex of DNA template and polymerase.
WO 90/13666 proposes a method directly measuring the growth of the template copy rather than determining it indirectly from compositions in the flow medium. Only one of the four nucleotides is present at a time, and the polymerisation events reflecting the incorporation of a nucleotide or not are detected by spectroscopic means (evanescent wave spectroscopy, fluorescence detection, absorption spectroscopy) or by the individual nucleotides being labelled.
Similar methods employing labelled 3 ' -blocked
deoxynucleotides where the blocking group is removable and which thus permit sequential deoxynucleotide
addition/detection steps are disclosed in WO 91/06678, US-A-5,302,509, DE-A-414 1178 and WO 93/21340. However, the necessary 3'-blocking groups are either not described in any detail, or are not accepted by the required enzyme, or do not permit desired rapid deblocking of the growing template copy strand after each polymerisation event.
One object of the present invention is to provide novel nucleotide derivatives which may be used as chain terminators and which by deprotection may readily be converted into nucleotides or nucleotide analogues that may be further extended.
Another object of the present invention is to provide a method for nucleotide sequence determination using the novel chain terminators.
Still another object of the present invention is to provide a method of synthesizing oligo- or polynucleotides by means of the novel chain terminators. Another object of the present invention is to provide a process of preparing novel chain terminators according to the invention.
In accordance with the invention, these objects are achieved by the provision of a chain terminating
nucleotide or nucleotide analogue having its 3'-hydroxyl group protected by an acetal or thioacetal structure designed in such a way that the 3'-hydroxyl can be
deprotected in a relatively short time in dilute acid, such as hydrochloric acid at pH 2, for example.
In one aspect, the present invention therefore provides a compound of the general formula I:
Figure imgf000006_0001
or a salt thereof, such as a trimethylammonium, ammonium, sodium or potassium salt, wherein
B is a nucleobase,
X and Z independently are oxygen or sulphur,
Y is hydrogen, hydroxy or protected hydroxy, such as methoxy, ethoxy or allyloxy,
R1 is hydrocarbyl, which optionally is substituted with a functional group,
R2 is hydrogen or hydrocarbyl, which optionally is substituted with a functional group,
A is an electron withdrawing or electron donating group capable of moderating the acetal stability of the compound I via L1, L1 and 1-2 are hydrocarbon linkers, which may be the same or different, L2, when present, being either (i) connected to L1 via the group A, or (ii) directly
connected to L1, the group A then being bound to one of linkers L1 and L2,
F is a dye label,
Q is a coupling group for F, and
1, m and n independently are O or 1, with the proviso that 1 is 1 when m is 1, and 1 is 1 and m is 1 when n is 1.
In Formula I above, the nucleobase B may be natural or synthetic. Natural nucleobases include common
nucleobases, such as adenine, guanine, cytosine, thymine and uracil, as well as less common nucleobases, such as xanthine, hypoxanthine or 2-aminopurine. Synthetic
nucleobases B are analogues to the natural nucleobases and capable of interacting with other nucleobases in a
specific, hydrogen bond determined way.
The hydrocarbyl groups represented by R1 and R2 include a wide variety, including straight and branched chain alkyl, alkenyl, aryl, aralkyl and cycloalkyl, preferably containing up to 10 carbon atoms. Preferred hydrocarbyl groups are primary, secondary or tertiary alkyl, alkenyl or alkynyl groups, especially lower alkyl groups, such as methyl and ethyl. The optional functional group substituents on R1 and R2 are capable of moderating the lability of the 3' acetal group through an inductive effect. Exemplary of such functional groups are tert.
amino, nitro, cyano and halogen (fluoride, chloride, bromide, iodide).
Detectable moiety, or label F can be chosen from a vast number of such moieties known to those skilled in the art. Exemplary such moities are radioactively labeled functions, luminescent, electroluminescent or fluorescent labels, and labels that absorb characteristic visible or infrared light. Preferably, F is a fluorescent label.
Coupling group Q, when n=0, is a reactive group to which a label F can be coupled, or, when n=1, is the derivatized residue of a reactive group used for coupling linker L2 to label F. A large number of such coupling groups capable of reacting with and binding label F via a reactive function thereon are known to those skilled in the art. Examples of reactive groups are amino, thio, and carboxyl. In some cases, the group Q is derived completely from the reactive function on the uncoupled F. For
example, if the coupling reaction is a substitution reaction, the group reacting with F being, for example, a halogen (fluoride, chloride, bromide or iodide), then the group Q will be represented by the reactive function present on label F.
For certain applications of the compounds of Formula I, as will be described below, no detectable moiety will be needed, and the label F, and optionally also the group Q, can then be omitted.
Electron withdrawing or donating group A is
incorporated into the structure as a moderator of acetal stability. The group A may represent a part of the chain L1-A-L2. Representative groups A in that case are amido, sulfoxy, sulfone, carbalkoxy (ester), ether, thioether and amino groups. Alternatively, A may be a side substituent for the L1-L2 chain, representative groups then being, for example, cyano, nitro and halogen (halogen including fluoride, chloride, bromide and iodide). In this latter case, linker L1 will donate structure stretching from the acetal carbon to the place of the substitution, and linker L2 will donate structure stretching from this substitution to the group A. It is to be emphasized that the specific electron withdrawing and electron donating groups
mentioned above are only examples and that many more such groups are known and obvious to those skilled in the art.
The structure of hydrocarbon linker L1 will be selected with regard to the function A, inductive effects being highly depending on distance. While a straight aliphatic (saturated or unsaturated) hydrocarbon chain is preferred, branched or cyclic hydrocarbons may be contemplated. Preferably, linker L1 has up to 10 carbon atoms, more preferably up to 6 carbon atoms.
The function of hydrocarbon linker L2 is to provide, together with linker L1, A and coupling group Q, for a sufficiently long distance between the label moiety F and the rest of the compound of Formula I. This is required by spatial preferences of the enzymes (polymerases) for which the compound of Formula I acts as substrate or by the necessity of avoiding interaction between the label and nucleobase B. It is readily understood that the structure of linker L2 highly depends on the particular enzyme, label F and possibly also nucleobase B that are used. A suitable length and structure of linker L2 will therefore be selected by the skilled person for each particular situation. Similarly as for linker L1, a preferred
structure for linker L2 is a straight aliphatic (saturated or unsaturated) hydrocarbon chain, although branched or cyclic hydrocarbons may be contemplated. Preferably, linker L2 has up to 10 carbon atoms, more preferably up to 6 carbon atoms.
In cases where the label F and the coupling group Q may be omitted, linker L2 may, of course, also be omitted.
The compounds of Formula I can be deprotected to exhibit a free 3'-hydroxy group in a relatively short time under acidic conditions, e.g. with hydrochloric acid at about pH 2. It is understood that by proper selection of the groups R1 , R2, A, L1 and L2 with regard to each other, the deprotection time may be adjusted to a desired range. Under the mentioned acidic conditions, the most preferred compounds of Formula I will be deprotected within, say, 0.01 to 15 minutes.
While the compounds of Formula I may be used as pure chain extension inhibitors, or chain terminators, for example, in DNA sequencing according to the chain
termination method, as is per se known in the art, the advantages of the compounds are, of course, better
benefited from when the convenient deprotection
capabilities of the compounds are utilized. This is, for example, the case when the compounds I are used in nucleic acid sequencing methods based on the sequential
incorporation and determination of individual nucleotides in a growing nucleic acid copy strand as described in, for example, the aforementioned WO 91/06678, US-A-5,302,509, DE-A-414 1178 and WO 93/21340.
Another aspect of the invention therefore provides a method for determining the sequence of a nucleic acid, which method comprises providing a single-stranded
template comprising the nucleic acid to be determined, and at least partially synthesizing a complementary nucleic acid molecule in a stepwise serial manner by the addition of nucleotides in which the identity of each nucleotide incorporated into the complementary nucleic acid molecule is determined subsequent to its incorporation, wherein said nucleotides are compounds of Formula I as defined above, and wherein the 3'-blocking group is removed from the nucleotide after its incorporation to permit further extension of the nucleic acid molecule.
In one embodiment, a method for determining the sequence of a nucleic acid comprises the following steps : (i) providing a single-stranded template comprising the nucleic acid to be sequenced,
(ii) hybridising a primer to the template to form a template/primer complex,
(iii) subjecting the primer to an extension reaction by the addition of compounds of Formula I with different nucleobases B corresponding the four bases A, C, T and G or analogues thereof,
(iv) determining the type of the compound of Formula I added to the primer,
(v) selectively hydrolysing the acetal protective group, and
(vi) repeating steps (iii) to (v) sequentially and recording the order of incorporation of compounds of
Formula I.
The different compounds of Formula I in step (iii) may be added in sequence, in which case the four different compounds I may carry the same label F. Alternatively, the different compounds I have different labels F and are added at the same time.
In a preferred embodiment of the method of the invention, the template/primer complex is bound to a solid-phase support, such as a sequencing chip, for example. The template may be attached to the solid support via a binding linker, which, for instance, is ligated to the 5'-end of the template or incorporated in one of the ends of the template by polymerase chain reaction (PCR). The binding linker may then be attached to the solid support by use of a streptavidin coupling system.
Alternatively, the primer may be attached to the solid support.
The compounds of Formula I may, of course, also conveniently be used in so-called mini-sequencing (see e.g. Syvanen A-C et al., Genomics 8:684-692 (1990).
As is readily understood by a person skilled in the art, the compounds of Formula I may also be used in the synthesis of nucleotide chains, and another aspect of the invention relates to such use. For example,
oligonucleotides and polynucleotides may be prepared by successively coupling compounds of Formula I to each other in any desired base order with intervening deblocking and using a non-template dependent polymerase, such as a terminal transferase. For such synthesis, the groups L2, Q and F in Formula I may, of course, be omitted.
The compounds of Formula I may be prepared by methods known per se. In a further aspect, however, the invention provides a particular method for the preparation of a subgroup of compounds of Formula I by direct 3'-OH
protection, and more particularly compounds of Formula Ia:
Figure imgf000012_0001
or a salt thereof, wherein B, X, Z, R1, R2, Q, F, m and n are as defined above, and p and q independently are integers from 1 to 10, preferably from 1 to 6 , by reacting a compound of Formula II:
Figure imgf000012_0002
or a salt thereof, wherein B and X are as defined above, with a compound of Formula III:
Figure imgf000012_0003
wherein R1 , R2, Z and p are as defined above , and R3 is hydrocarbyl ( for example , as def ined for R1 and R2 above) , to produce a compound of Formula IV:
Figure imgf000012_0004
or a salt thereof, wherein B, X, Z, R1, R2, R3 and p are as defined above, optionally reacting the latter with a diamine H2N-(CH2)q-NH2, wherein q is as defined above, to produce a compound of Formula V:
Figure imgf000013_0001
wherein B, X, Z, R1, R2, p and q are as defined above, and optionally coupling a dye label F to the terminal amino group.
In the following, the invention will be illustrated by some non-limiting examples. Reference will be made to the accompanying drawings, wherein:
Fig. 1 is a reaction scheme for the enolether
synthesis described in Example 1 below. Intermediate and final products corresponding to various values of integer "n" in the respective structural formulae are identified by numbers indicated within brackets after the n-values listed under the respective formulae.
Fig. 2 is a reaction scheme for the preparation of 3'-acetal-modified thymidine described in Example 2 below. Prepared final compounds corresponding to various values of integer "n" in the respective structural formula are identified by numbers indicated within brackets after the n-values listed under the formula.
Fig. 3 is a graph showing thymidine 3'-acetal
hydrolysis at pH 4 as log % of remaining acetal versus time in minutes.
Fig. 4 is a reaction scheme for the one-pot synthesis of 3'-acetal protected deoxynucleotide triphosphates described in Example 4 below. Intermediate and final products corresponding to various values of integer "n" in the respective structural formulae are identified by numbers indicated within brackets after the n-values listed under the respective formulae.
EXAMPLE 1
Synthesis of enolethers for derivatization of nucleotide triphosphates (Fig. 1)
Step 1. Esterification of ketoacids
The appropriate ketoacid (1 eq) was added at once to a large excess of dry methanol (20 eq), previously treated with thionyl chloride (0.1 eq). The homogenous mixture was refluxed overnight, evaporated under reduced pressure, and partitioned between saturated sodium hydrogen carbonate and dichloromethane. The combined organic extracts were dried with magnesium sulphate, evaporated and the residue was distilled under reduced pressure to give the
appropriate methyl ester in a high yield (80% to 95%) .
The following ketoacids were used:
1) 4-oxy pentanoic acid (levulinic acid) (Aldrich)
2) 5-oxy hexanoic acid has not been isolated. Instead a commercial ethyl ester-derivative of this acid (Merck) was transesterified in a reaction analogous to the above general procedure.
3) 6-oxy heptanoic acid was obtained from 2-methyl cyclohexanol (Merck), according to a published procedure (Org. Synth. 31: 3-5, (1951)).
4) 7-oxy octanoic acid was obtained from 2-acetyl cyclohexanone as described (J. Am. Chem. Soc. 70:4023-4026 (1948)).
Step 2. Synthesis of the dimethoxvacetal derivatives
(compounds 1-4 in Fig. 1)
Benzenesulfonic acid (0.01 eq) was added to each of above methyl esters (1 eq) dissolved in methanol (2 eq) and trimethylorthoformate (3 eq). The dark brown mixture was refluxed for 3 h, neutralized by addition of dry triethylamine (0.1 eq), and evaporated. The residue was distilled under lowered pressure to yield a pure acetal. Compound 1. The physical and NMR data for this acetal correspond well to the data reported previously.
Compound 2. Yield 85%, bp. 120° (15 mm Hg) 1H NMR (CDCl3): 1.28 (s, 3 H), 1.60-1.69 (m, 4 H), 2.34 (t, 2 H), 3.17 (s, 6 H) , 3.67 (s, 3 H).
Compound 3. Yield 92%, bp. 130-133° (15 mm Hg) 3-H NMR (CDCI3): 1.25 (s, 3 H) , 1.29-1.35 (m, 2 H), 1.60-1.70 (m, 4 H), 2.33 (t, 2 H), 3.17 (s, 6 H), 3.67 (s, 3 H).
Compound 4. Yield 87%, bp. 147-149° (15 mm Hg) 1H NMR (CDCI3): 1.25 (s, 3 H), 1.27-1.38 (m, 4 H), 1.57-1.67 (m, 4 H), 2.31 (t, 2 H), 3.16 (s, 6 H), 3.66 (s, 3 H).
Step 3. Synthesis of enolethers (compounds 5-8 in Fig. 1).
A mixture of the appropriate acetal (1 eq) and trimethylortoformate (0.5 eq) was placed in a distillation flask, equipped with a 20 cm Vigreux column.
Benzenesulfonic acid (0.02 eq) was added and the mixture was refluxed. The heating was regulated so that the liberated methanol evaporated slowly. After 4 h the heating was increased and the dark mixture was
fractionated under reduced pressure without previous neutralization of the acidic catalyst. The yields of isolated colorless enolethers were in all cases very high (85-95%) but GC and NMR analyses showed the presence of starting acetal in proportions from 10 to 30 %. Since these impurities were not expected to influence the derivatization of nucleotides no attempts were made to purify them further. The complete assignment of NMR signals was difficult because of the presence of starting material and the fact that these asymmetric enolethers exist as several isomeric forms. Nevertheless, in all spectra a vinylic signal of CH2 from one isomer at around 4.4 to 4.5 ppm and a vinylic signal of CH from the other isomer at 3.85 ppm could be easily observed. EXAMPLE 2
Synthesis of 3' acetal-modified thymidine (Fig. 2)
The 5'-protected thymidine, 5'-FMOC T (FMOC-fluorenyl methoxycarbonyl), (116 mg, 0.25 mmol) was dried by
coevaporation with dry acetonitrile (10 ml) and dissolved in dry dioxane (5 ml). To this magnetically stirred solution an appropriate enolether (0.5 ml, = 10 eq) prepared in Example 1 was added, followed by
trifluoroacetic acid (20 ml, 1 eq). After 45 min, the TLC analysis (Silicagel 60 F254, 10% methanol in chloroform) showed complete consumption of the starting material, and dry triethylamine (2 ml) was introduced in order to remove the base-labile FMOC-group. After this process was
completed (60 min), the whole mixture was evaporated under reduced pressure. The nucleoside was separated from the excess of enolether by precipitation from petroleum ether, and the precipitate, dissolved in 5 ml of dry methanol, was treated with 1,3-diaminopropane (2 ml, 100 eq) at 60° for 180 min in order to effect the aminolysis of the ester function on the acetal moiety. Finally, the reaction mixture was evaporated under low pressure (oil pump) and the crude material was flash chromatographed on a silica gel column, equilibrated in ethanol and using a step gradient of cone, ammonium hydroxide (0-10%) in ethanol. The material, homogeneous by TLC (developed in 1-butanol -ammonium hydroxide 8:2), was combined, evaporated, and coevaporated with toluene, to give the NMR pure product (compounds 9-12 in Fig. 2) in high yield (72 to 85%) . The pure material was stored as a stock solution in methanol after addition of three drops of ammonia.
EXEMPLE 3
Acidic hydrolysis (pH 4) of thymidine, substituted at the
3'-position with different acetyl groups A reference acetate buffer pH 4.0, prepared by mixing of solutions of sodium acetate (0.20 M, 18.0 ml) with acetic acid (0.20 M, 82.0 ml) was used in all hydrolysis studies. To this buffer (10.0 ml) an ethanolic solution of the appropriate thymidine 3'-acetal derivative prepared in Example 2 (compounds 9-12 in Fig. 2) (100 ml) was added with gentle stirring. At different time points a sample of 0.5 ml was withdrawn and placed in a tube containing 15 ml of cone ammonia to raise the pH to 9. Samples were analyzed by FPLC using an anion exchange column (Mono Q - Pharmacia Biotech AB) and a gradient system of
tetraethylammonium bicarbonate pH 8.2 for elution (0.05 to 0.75 M). The peak areas of starting material and its hydrolysis product thymidine were integrated, and plotted as shown in Fig. 3.
EXAMPLE 4
One pot-synthesis of deoxynucleotide triphosphates, protected at their 3'-OH position by a functionalized acetal group (Fig. 4)
A commercial deoxynucleotide triphosphate (pppdT, pppdC, pppdG, or pppdA) was chromatographed on a
preparative Mono Q column using a gradient system of tetraethylammonium bicarbonate pH 8.2 (0.05 to 1.3 M) to obtain the pure triphosphate in the form of a
triethylammonium salt. This material was evaporated on a Rotavapor, coevaporated with dry acetonitrile (3×2 ml), and dissolved in molecular sieve-dried trimethylphosphate (0.5 ml). The appropriate enolether (compounds 5-8 in Fig. 1) (0.2 ml) and trifluoroacetic acid (10 eq as a 10% solution in dry dioxane) were added. The homogeneous mixture was incubated at 20°C for 60 min, neutralized by the addition of triethylamine (100 ml), and precipitated from a 1:1 mixture of petroleum ether and diethyl ether. The oily precipitate was dissolved in methanol (2 ml) and 1,3-diaminopropane (0.5 ml) or another diamine (1,4-diaminobutane, 1,6-diaminohexane) (0.5 ml) was added. The ester function was subjected to aminolysis overnight at 60°C. The mixture was again precipitated from 1:1
petroleum ether and diethyl ether, washed with diethyl ether, and dissolved in water. The water solution was analyzed and preparatively purified on the described anion exchange column. The well resolved products (compounds 13-28 in Fig. 4) always appear prior to the original deoxynucleotide triphosphate, having a retention time comparable to that of the appropriate deoxynucleotide diphosphate (as was found from separate coinjection experiments). An aliquot of the isolated 3'-acetal-modified derivative was evaporated, treated with 80% acetic acid for 2 min, and, after evaporation of acid, reinjected to the same chromatographic system. In all cases all starting material was reacted and a single product with higher retention time was formed that
corresponded to the original deoxynucleotide triphosphate. Thymidine triphosphate reacts to form, besides the desired 3' -modified derivative, also another product with even shorter retention time but that also hydrolyses to the starting triphosphate during acid treatment. It is assumed that this product is the bis-3'-O, 4-O-acetal-derivative of thymidine triphosphate. This type of side products was not present in reactions that used other nucleotide triphosphates. It should also be stressed that very little products of depurination were formed in reactions in which pppdG and pppdA were used. This can be explained by the mild acid applied as a catalyst, the large excess of enolether used in the reaction, and the fact that the bases existed in an unprotected (more acid resistant) form.
EXAMPLE 5
Coupling of a fluorophore to the 3'-functionalised
deoxynucleotide triphosphate (Fig. 4) This derivatization can be performed with a variety of reactive fluorophores that may differ in their
reactivity and in their optimal reaction conditions. Here is described the procedure for labelling of 3'-functionalized deoxynucleotide triphosphate with
fluorescein isothiocyanate.
The appropriate nucleotide triphosphate, possessing an amino group attached to the 3'- position of the sugar residue via an acetal function (compounds 13-28 in Fig. 4), was evaporated and dissolved in 0.1 M carbonate buffer pH 10 (0.5 ml). Fluorescein isothiocyanate (single isomer) (10 eq), dissolved in dimethylformamide (0.25 ml), was added and the mixture was incubated overnight at 20°C. The reaction mixture was applied on a prototype FPLC Superdex® gel filtration column (Pharmacia Biotech AB) (equivalent to Sephadex® G-10; Pharmacia Biotech AB), equilibrated and run in TEA HCO3 buffer (0.1 M). The fluorescent material appearing in the void was collected (compounds 29-44 in Fig. 4). As expected, the original deoxynucleotide
triphosphate was formed upon action of acid on the
fluorescein-labelled nucleotide.
EXAMPLE 6
Stepwise enzymatical incorporation of 3'-modified
triphosphates
Four oligonucleotides were prepared, having sequences corresponding to the M13 sequencing primer, and designed to incorporate to their 3'-ends T, G, A or C base
respectively :
Figure imgf000019_0001
Each of them was rad oact vely labelled with 32P using T4 polynucleotidekinase.
In order to investigate if the modified nucleotide triphosphates are accepted effectively and specifically by the T7 polymerase, each of the labelled primers was subjected to the single step extension conditions. These reaction mixtures (20 ml) were composed of the respective primer (0.1 pmol), M13 template (1 pmol), and 3'-modified thymidine triphosphate (compound 16 in Fig. 4) in a buffer system pH 7.5 containing Tris/HCl (40 mM), MnCl2 (4 mM), dithiothreitol (DTT) (11 mM), sodium isocitrate (29 mM) and sodium chloride (23 mM). The mixtures were denatured at 70°C, cooled, and incubated at 42°C after the addition of T7 DNA polymerase (10 U) for 30 min. All reactions were stopped by addition of formamide (20 ml), denatured at 70°C, cooled on ice, and separated on a 6% denaturing sequencing gel . The developed autoradiogram showed that one-base extension had taken place solely in the reaction containing 23-mer-T (designed to prime the M13 template and incorporate thymidylic acid at its 3'-end). None of the other reactions containing primers designed for incorporation of dG, dA and dC, respectively, showed any sign of primer extension.
EXAMPLE 7
Sequencing reaction with modified chain terminator All sequencing reactions were performed according to the standard ABI protocol (Taq Dye Primer Cycle Sequencing Kit - protocol 901482).
The sequencing reactions consisted of the following components: M13 mp 18 ss-DNA template (1 pmol), 5'-fluorescein labelled universal primer (1 pmol, Pharmacia Biotech AB), Ampli Taq DNA polymerase (4U) and T-termination mixture in cycle sequencing buffer (Tris-HCl pH 8.9, 80 mM, ammonium sulfate 20 mM, magnesium chloride 5 mM). Instead of the standard ddT triphosphate, compound 16 in Fig. 4, in different proportions with TTP, was used as a chain terminator. After the cycling was completed, an equal volume of formamide was added and the mixture was heated for 2 min at 90°C, cooled on ice and loaded onto 6% acrylamide urea gel. Separation and analysis of products were performed on an A.L.F. DNA-sequencer (Pharmacia
Biotech AB).
As a result, a pattern of fluorescent-labelled sequences was obtained. This electrophoretic picture was specific for the applied terminator.

Claims

A compound of the general structure I:
Figure imgf000021_0001
or a salt thereof, wherein
B is a nucleobase,
X and Z independently are oxygen or sulphur,
Y is hydrogen or hydroxy, which optionally may be protected,
R1 is hydrocarbyl, which optionally is substituted with a functional group,
R2 is hydrogen or hydrocarbyl, which optionally is substituted with a functional group,
A is an electron withdrawing or electron donating group capable of moderating the acetal stability of the compound I,
L1 and L2 are hydrocarbon linkers, which may be the same or different, L2, when present, being either (i) connected to L1 via the group A, or (ii) directly
connected to L1, the group A then being connected to one of linkers L1 and L2,
F is a dye label,
Q is a coupling group for F, and
1, m and m independently are 0 or 1, with the proviso that 1 is 1 when m is 1, and 1 is 1 and m is 1 when n is 1.
2. The compound according to claim 1, wherein R1 and R2 are independently selected from primary, secondary and tertiary alkyl, optionally substituted with one or more functional groups.
3. The compound according to claim 2, wherein R1 and R2 are selected from methyl and ethyl.
4. The compound according to claim 1, 2 or 3, wherein A is a part of a chain L1-A-L2 and is selected from amido, sulfoxy, sulfone, carbalkoxy, ether, thioether and amino.
5 . The compound according to claim 1, 2 or 3, wherein A is a substituent to a chain L1-L2 and is selected from cyano, nitro and halogen.
6. The compound according to any one of claims 1 to 5, wherein L1 is a straight aliphatic hydrocarbon chain, preferably having up to 10 carbon atoms.
7. The compound according to any one of claims 1 to 6 , wherein L2 is a straight aliphatic hydrocarbon chain, preferably having up to 10 carbon atoms.
8. The compound according to any one of claims 1 to 7, wherein Y is alkoxy.
9. Use of compounds according to any one of claims 1 to 8 in nucleic acid synthesis reactions, especially for preparing oligo- or polynucleotides.
10. Use of compounds according to any one of claims 1 to 8 in minisequencing.
11. A method for determining the sequence of a nucleic acid, comprising providing a single-stranded template comprising the nucleic acid to be determined, and at least partially synthesizing a complementary nucleic acid molecule in a stepwise serial manner by the addition of nucleotides in which the identity of each nucleotide incorporated into the complementary nucleic acid molecule is determined subsequent to its incorporation, wherein said nucleotides are compounds of Formula I as defined in any one of claims 1 to 8, and wherein the 3'-blocking group is removed from the nucleotide after its
incorporation to permit further extension of the nucleic acid molecule.
12. The method according to claim 11, wherein the 3'-blocking group is removed by acid hydrolysis.
13. The method according to claim 11 or 12, wherein F in Formula I is a fluorescent label.
14. The method according to any one of claims 11 to 13, wherein said single-stranded template is bound to a solid support.
15. A process of preparing a compound of Formula la:
Figure imgf000023_0001
ar a salt thereof, wherein B, X, Z, R1, R2, Q, F, m and n are as defined in claim 1, and p and q independently are integers from 1 to 10, by reacting a compound of Formula II:
Figure imgf000024_0003
or a salt thereof, wherein B and X are as defined above, with a compound of Formula III:
Figure imgf000024_0004
wherein R1, R2, Z and p are as defined above, and R3 is hydrocarbyl, to produce a compound of Formula IV:
Figure imgf000024_0001
or a salt thereof, wherein B, X, Z, R1, R2, R3 and p are as defined above, optionally reacting the latter with a diamine H2N-(CH2)q-NH2, wherein q is as defined above, to produce a compound of Formula V:
Figure imgf000024_0002
wherein B, X, Z, R1, R2, p and q are as defined above, and optionally coupling a dye label F to the terminal amino group.
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US6255475B1 (en) 2001-07-03
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SE9500342D0 (en) 1995-01-31

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