Patent Application: US-27098305-A

Abstract:
the detection of specific dna sequences using electrochemical readout would permit the rapid and inexpensive detection and identification of bacterial pathogens and the analysis of human genes . a new assay developed for this purpose is described that harnesses an electrocatalytic process to monitor dna hybridization .

Description:
the invention relates to a new electrocatalytic nucleic acid detection assay that reports nucleic acid hybridization between a nucleic acid probe and a nucleic acid , or between a first nucleic acid and a second nucleic acid , and can resolve single - base changes in a target nucleic acid sequence . the method exploits a reaction between a redox pair comprising a first redox - active probe ( i . e ., a nucleic acid - binding compound ) and a second redox - active probe . the nucleic acid - binding compound comprises a redox active compound that can bind to the nucleic acid electrostatically and can be reduced at low potential . this compound is bound to the nucleic acid , producing an electrostatically bound complex . the signal generated by the binding can be amplified by use of a redox active probe that can reoxidize the electrostatically bound complex . “ solid support ”, as used herein , refers to the material to which the nucleic acid probe is attached . suitable solid supports are available commercially , and will be apparent to the skilled person . the supports can be manufactured from materials such as glass , ceramics , silica and silicon , and can incorporate conductive material to serve as an electrode . conductive supports with a gold surface may also be used . the supports usually comprise a flat ( planar ) surface , or at least a structure in which the polynucleotides to be interrogated are in approximately the same plane . the support can be an electrode , or can be attached to an electrode . “ mismatch ”, as used herein , refers to a duplex in which less than all of the nucleotides on one strand are perfectly matched to the other strand ( e . g ., where nucleotide pairing other than adenosine - thymine or guanine - cytosine occurs , e . g ., nucleotide paring such as adenosine - cytosine , adenosine - guanine , adenosine - adenosine , thymine - cytosine , thymine - guanine , thymine - thymine , guanine - guanine , or cytosine - cytosine occurs ), where a deletion or insertion of one or more dna nucleotides on one strand as compared to the other complementary strand occurs ( e . g ., a deletion of 1 , 2 , 5 , 10 , 15 , or more nucleotides or an insertion of 1 , 2 , 5 , 10 , 15 , or more nucleotides occurs ), or other mismatches between the two strand of the duplex occurs . dna mismatches may arise from nucleic acid replication errors , mutagenesis , deamination of 5 - methylcytosine , formation of thymidine dimers , nucleic acid recombination , etc . by “ probe ” is meant a single - stranded oligonucleotide capable of binding to at least a portion of the target nucleic acid sought to be detected . the probe will generally have a sequence partly or completely complementary to a target nucleic acid sequence sought to be detected , so as to stably hybridize thereto under stringent hybridization conditions . in the case of a group or species - specific probe , the probe has the ability to stably hybridize to a target nucleic acid and not to non - target nucleic acids such as those from organisms outside the phylogenetic group or species under stringent hybridization conditions . probes may , but need not , have regions which are not complementary to a target sequence , as long as such sequences do not substantially alter the probe &# 39 ; s desired specificity under stringent hybridization conditions . as used herein , the term “ a nucleic acid probe ” also refers to a nucleic acid capable of binding to a target nucleic acid of complementary sequence through one or more types of chemical bonds , usually through complementary base pairing , usually through hydrogen bond formation . as used herein , a probe may include natural ( i . e ., a , g , c , or t ) or modified on bases ( 7 - deazaguanosine , inosine , etc .) or on sugar moiety . in addition , the bases in a probe can be joined by a linkage other than a phosphodiester bond , so long as it does not interfere with hybridization . thus , for example , probes can be peptide nucleic acids in which the constituent bases are joined by peptide bonds rather than phosphodiester linkages . it will be understood by one of skill in the art that probes may bind target sequences lacking complete complementarity with the probe sequence depending upon the stringency of the hybridization conditions . by assaying for the presence or absence of the probe , one can detect the presence or absence of the select sequence or subsequence . as used herein , the term “ nucleic acid ” refers to polynucleotides such as deoxyribonucleic acid ( dna ), and , where appropriate , ribonucleic acid ( rna ). the term should also be understood to include , as equivalents , analogs of either rna or dna made from nucleotide analogs , and , as applicable to the embodiment being described , single ( sense or antisense ) and double - stranded polynucleotides . ests , chromosomes , cdnas , mrnas , and rrnas are representative examples of molecules that can be referred to as nucleic acids . as used herein , the term “ hybridization ” refers to any process by which a strand of nucleic acid binds with a complementary strand through base pairing . as used herein , the term “ hybridization conditions ” refer to standard conditions under which nucleic acid molecules are used to identify similar nucleic acid molecules . such standard conditions are disclosed , for example , in sambrook et al ., molecular cloning : a laboratory manual , cold spring harbor labs press , 1989 . sambrook et al ., ibid ., is incorporated by reference herein in its entirety ( see specifically , pages 9 . 31 - 9 . 62 ). in addition , formulae to calculate the appropriate hybridization and wash conditions to achieve hybridization permitting varying degrees of mismatch of nucleotides are disclosed , for example , in meinkoth et al ., 1984 , anal . biochem . 138 , 267 - 284 ; meinkoth et al ., ibid ., is incorporated by reference herein in its entirety . non - limiting examples of hybridization conditions include low stringency hybridization conditions , moderate stringency hybridization conditions and high stringency hybridization conditions . as used herein , the term “ sample ” as used in its broadest sense , refers to any plant , animal or viral material containing dna or rna , such as , for example , tissue or fluid isolated from an individual ( including without limitation plasma , serum , cerebrospinal fluid , lymph , tears , saliva and tissue sections ) or from in vitro cell culture constituents , as well as samples from the environment . the sample of nucleic acids can be drawn from any source and can be natural or synthetic . the sample of nucleic acids may contain of deoxyribonucleic acids ( dna ), ribonucleic acids ( rna ), or copolymers of deoxyribonucleic acids and ribonucleic acids or combinations thereof . alternatively , the sample may have been subject to purification ( e . g . extraction ) or other treatment . the term “ sample ” can also refer to “ a biological sample .” as used herein , the term “ a biological sample ” refers to a whole organism or a subset of its tissues , cells or component parts ( e . g . body fluids , including but not limited to blood , mucus , lymphatic fluid , synovial fluid , cerebrospinal fluid , saliva , amniotic fluid , amniotic cord blood , urine , vaginal fluid and semen ). “ a biological sample ” further refers to a homogenate , lysate or extract prepared from a whole organism or a subset of its tissues , cells or component parts , or a fraction or portion thereof , including but not limited to , for example , plasma , serum , spinal fluid , lymph fluid , the external sections of the skin , respiratory , intestinal , and genitourinary tracts , tears , saliva , milk , blood cells , tumors , organs . most often , the sample has been removed from an animal , but the term “ biological sample ” can also refer to cells or tissue analyzed in vivo , i . e ., without removal from animal . typically , a “ biological sample ” will contain cells from the animal , but the term can also refer to non - cellular biological material , such as non - cellular fractions of blood , saliva , or urine , that can be used to measure the cancer - associated polynucleotide or polypeptides levels . “ a biological sample ” further refers to a medium , such as a nutrient broth or gel in which an organism has been propagated , which contains cellular components , such as proteins or nucleic acid molecules . as used herein , the term “ an increase of the signal ” means that the signal generated from hybridization between two nucleic acids is greater than that generated from either one of said two nucleic acids alone in unhybridized form . preferably , the hybridization is between a nucleic acid probe and a target nucleic acid . also preferably , the hybridization is between a first nucleic acid and a second nucleic acid . preferably , the increase is at least about 10 %, preferably at least about 15 %, about 25 %, about 30 %, about 40 %, about 50 %, about 65 %, about 75 %, about 85 %, about 90 %, about 95 %, about more than 100 %, about twofold , about ten fold , about fifty fold , or greater . as used herein , the term “ decrease of the signal ” means that the signal generated from hybridization between two nucleic acids that are complementary but for a mismatch , is lower than that generated from hybridization between two completely complementary nucleic acids . preferably , the decrease is at least about 10 %, preferably at least about 15 %, about 25 %, about 30 %, about 40 %, about 50 %, about 65 %, about 75 %, about 85 %, about 90 %, about 95 %, about more than 100 %, about twofold , about ten fold , about fifty fold , or greater . as used herein , the term “ a transition metal ” refers to any of the elements found between the group iia elements and the group iib elements in the periodic table . transition metals to be used in a transition metal complex of the present invention include those of the fourth , fifth , and sixth periods of the periodic table of elements . preferably , the transition metals used in the present invention include iron , ruthenium , cobalt , molybdenum , osmium and rhenium . as used herein , the term “ transition metal complex ” refers to a structure composed of a central transition metal atom or ion , generally a cation , surrounded by a number of negatively charged or neutral ligands possessing lone pairs electrons that can be given to the central metal . the transition metal is defined herein above . the ligands bind to the central transition metal using dative bonds . there are a number of different types of ligands that can be applied to the present invention . non - limiting examples include but not limited to , monodentate ligands , bidendate ligands , tridendate ligands , tetradentate ligands and hexadentaate ligands , etc . preferably , the ligands can be pyridine - based , phenathroline - based , heterocyclic , aquo , aromatic , chloride ( cl − ), or ammonia ( nh 3 ), or cyanide ( cn − ). described herein is an electrocatalytic detection assay that reports hybridization between nucleic acids , or between nucleic acids and proteins . in one aspect , the assay can be used to detect hybridization between a nucleic acid probe and a dna or rna target . the present assay is sufficiently sensitive to resolve single - base changes in the target sequence . the method exploits a reaction between a redox pair comprising a nucleic acid - binding compound and a redox - active probe . the nucleic acid - binding compound can be a transition metal complex . preferably , the transition metal is one selected from the group consisting of cobalt , iron , molybdenum , osmium , ruthenium and rhenium . also preferably , the transition metal complex is an ammonium complex of the transition metal . more preferably , the transition metal complex is ru ( nh 3 ) 6 3 + . the redox active probe can also be a transition metal complex . preferably , the transition metal is one selected from the group consisting of cobalt , molybdenum , osmium , iron and rhenium . also preferably , the transition metal complex is a cynate complex of the transition metal . more preferably , the transition metal complex is fe ( cn ) 6 − 3 . the nucleic acid - binding compound binds to the nucleic acid primarily through electrostatic interactions with the phosphate backbone , and therefore its electrochemical reduction yields a signal that reports on the increase of negatively charged groups at the electrode surface upon hybridization of a target nucleic acid . the signal is amplified by the transition metal oxidant of the redox active probe which permits the transition metal to be regenerated for multiple cycles . the immobilization of the nucleic acid probe on highly conductive surfaces , e . g ., gold , amplifies the kinetic effects of base mismatches on nucleic acid hybridization , permitting single - base changes to be resolved . one advantage of the assay is the use of the nucleic acid - binding compound to report the hybridization event and the coupling of this signal to an electrocatalytic process . the design also provides superior sensitivity , e . g ., detection of a single base mismatch . the invention described herein is useful for the detection of infectious bacterial and viral agents . the invention is also useful in detecting genes and proteins , e . g ., changes in genes and proteins , e . g ., changes in oncogenes . it therefore is useful in a clinical diagnostic setting , and for detection of pathogenic agents in non - clinical settings , e . g ., detection of bioterror agents . in another aspect , the method described herein can be used to determine the presence of a target nucleic acid according to the following protocol . a biological sample suspected of containing the target nucleic acid may optionally be treated to release any nucleic acid contained within the sample . for instance , the sample can be serum , blood , other bodily fluids , tissue , etc . the sample can also be from a human , an animal , a plant , etc . the sample can also be nucleic acid washed from a swab or some other type of material used to wipe surfaces to detect contaminants . the sample can also be nucleic acid extracted or washed off of a filter through which air is passed , e . g . a filter from an air filtration system , in the case of detecting airborne bioterror agents . such an article can be treated to extract the nucleic acid by methods that are known in the art , e . g ., forensics and contamination detection . the nucleic acid extracted from the article can be tested directly by the methods described herein , or can be amplified to enhance detection . in one embodiment , the invention features a method of detecting nucleic acid hybridization between a nucleic acid probe and a target nucleic acid in a sample , where the method includes the steps of : ( a ) providing a nucleic acid probe immobilized on a solid substrate ; ( b ) contacting , under hybridizing conditions , the solid support and the immobilized probe to a solution containing the sample and a redox pair , wherein the redox pair comprises a first transition metal complex and a second transition metal complex ; and ( c ) measuring the electrocatalytic signal generated by hybridization of the nucleic acid probe and the target nucleic acid ; where an increase of the signal detected in step ( c ) relative to that of a control sample containing no nucleic acid , indicates that the nucleic acid hybridization has occurred . the method can also include an additional step of testing a control , by contacting , under hybridizing conditions , the solid support and the immobilized nucleic acid probe to a solution containing no sample , and a redox pair comprising a first transition metal complex and a second transition metal complex . preferably , the transition metal of the first transition metal complex is one selected from the group consisting of cobalt , iron , molybdenum , osmium , ruthenium and rhenium . more preferably , the transition metal of the first transition metal complex is ruthenium . also preferably , the first transition metal complex is a transition metal ammonium complex . more preferably , the first transition metal ammonium complex comprises a transition metal selected from the group consisting of cobalt , iron , molybdenum , osmium , ruthenium and rhenium . most preferably , the transition metal ammonium complex is ru ( nh 3 ) 6 3 + . preferably , the transition metal of the second transition metal complex is one selected from the group consisting of cobalt , molybdenum , osmium and rhenium . more preferably , the transition metal of the second transition metal complex is iron . also preferably , the second transition metal complex is a transition metal cynate complex . more preferably , the second transition metal cynate complex comprises a transition metal selected from the group consisting of cobalt , molybdenum , osmium and rhenium . most preferably , the second transition metal cynate complex is fe ( cn ) 6 − 3 . in another embodiment , the invention also features a method of detecting nucleic acid hybridization between a first nucleic acid and a second nucleic acid , wherein the method includes the steps of : ( a ) providing the first nucleic acid immobilized on a solid support ; ( b ) contacting , under hybridizing conditions , the solid support and the immobilized first nucleic acid to a solution suspected of containing the second nucleic acid and a redox pair comprising a first transition metal complex and a second transition metal complex ; and ( c ) measuring the electrocatalytic signal generated by hybridization of the first and second nucleic acids ; wherein an increase of the signal detected in step ( c ) relative to that of an unhybridized first nucleic acid , indicates that nucleic acid hybridization has occurred . the method can also include an additional step of testing a control , by contacting , under hybridizing conditions , the solid support and the immobilized first nucleic acid to a solution containing no sample , and a redox pair comprising a first transition metal complex and a second transition metal complex . preferably , the transition metal of the first transition metal complex is one selected from the group consisting of cobalt , iron , molybdenum , osmium , ruthenium and rhenium . more preferably , the transition metal of the first transition metal complex is ruthenium . also preferably , the first transition metal complex is a transition metal ammonium complex . more preferably , the first transition metal ammonium complex comprises a transition metal selected from the group consisting of cobalt , iron , molybdenum , osmium , ruthenium and rhenium . most preferably , the transition metal ammonium complex is ru ( nh 3 ) 6 3 + . preferably , the transition metal of the second transition metal complex is one selected from the group consisting of cobalt , molybdenum , osmium and rhenium . more preferably , the transition metal of the second transition metal complex is iron . also preferably , the second transition metal complex is a transition metal cynate complex . more preferably , the second transition metal cynate complex comprises a transition metal selected from the group consisting of cobalt , molybdenum , osmium and rhenium . most preferably , the second transition metal cynate complex is fe ( cn ) 6 − 3 . in another aspect , the invention features a method of detecting a mismatch between a first nucleic acid and a second nucleic acid , comprising : ( a ) providing a nucleic acid probe immobilized on a solid support ; ( b ) contacting , under hybridizing conditions , the solid support and the immobilized probe to a solution containing the sample containing a target nucleic acid and a redox pair , wherein the redox pair comprises a first transition metal complex and a second transition metal complex ; and ( c ) measuring the electrocatalytic signal generated by hybridization of the nucleic acid probe and the target nucleic acid ; wherein a decrease of the signal detected in step ( c ) relative to that of a perfect complementarity between the nucleic acid probe and the target nucleic acid , indicates that there is a mismatch between the first nucleic acid and the second nucleic acid . the method can also include an additional step of testing a control , by contacting , under hybridizing conditions , the solid support and the immobilized nucleic acid probe to a solution containing no sample , and a redox pair comprising a first transition metal complex and a second transition metal complex . preferably , the transition metal of the first transition metal complex is one selected from the group consisting of cobalt , iron , molybdenum , osmium , ruthenium and rhenium . more preferably , the transition metal of the first transition metal complex is ruthenium . also preferably , the first transition metal complex is a transition metal ammonium complex . more preferably , the first transition metal ammonium complex comprises a transition metal selected from the group consisting of cobalt , iron , molybdenum , osmium , ruthenium and rhenium . most preferably , the transition metal ammonium complex is ru ( nh 3 ) 6 3 + . preferably , the transition metal of the second transition metal complex is one selected from the group consisting of cobalt , molybdenum , osmium and rhenium . more preferably , the transition metal of the second transition metal complex is iron . also preferably , the second transition metal complex is a transition metal cynate complex . more preferably , the second transition metal cynate complex comprises a transition metal selected from the group consisting of cobalt , molybdenum , osmium and rhenium . most preferably , the second transition metal cynate complex is fe ( cn ) 6 − 3 . the invention additionally features a method of detecting a mismatch between a first nucleic acid and a second nucleic acid , wherein the method includes the following steps : ( a ) providing the first nucleic acid immobilized on a solid support ; ( b ) contacting , under hybridizing conditions , the solid support and the immobilized first nucleic acid to a solution containing the sample containing the second nucleic acid and a redox pair , wherein the redox pair comprises a first transition metal complex and a second transition metal complex ; and ( c ) measuring the electrocatalytic signal generated by hybridization of the first nucleic acid and the second nucleic acid ; wherein a decrease of the signal detected in step ( c ) relative to that of a perfect complementarity between the first nucleic acid and the second nucleic acid , indicates that there is a mismatch between the first nucleic acid and the second nucleic acid . the method can also include an additional step of testing a control , by contacting , under hybridizing conditions , the solid support and the immobilized nucleic acid probe to a solution containing no sample , and a redox pair comprising a first transition metal complex and a second transition metal complex . preferably , the transition metal of the first transition metal complex is one selected from the group consisting of cobalt , iron , molybdenum , osmium , ruthenium and rhenium . more preferably , the transition metal of the first transition metal complex is ruthenium . also preferably , the first transition metal complex is a transition metal ammonium complex . more preferably , the first transition metal ammonium complex comprises a transition metal selected from the group consisting of cobalt , iron , molybdenum , osmium , ruthenium and rhenium . most preferably , the transition metal ammonium complex is ru ( nh 3 ) 6 3 + . preferably , the transition metal of the second transition metal complex is one selected from the group consisting of cobalt , molybdenum , osmium and rhenium . more preferably , the transition metal of the second transition metal complex is iron . also preferably , the second transition metal complex is a transition metal cynate complex . more preferably , the second transition metal cynate complex comprises a transition metal selected from the group consisting of cobalt , molybdenum , osmium and rhenium . most preferably , the second transition metal cynate complex is fe ( cn ) 6 − 3 . in another embodiment , the invention also features a method of detecting nucleic acid hybridization between a nucleic acid probe and a target nucleic acid , where the method includes the following steps : ( a ) providing a nucleic acid probe immobilized on a solid support ; ( b ) contacting the immobilized probe to a solution containing : ( i ) a transition metal complex ; ( c ) measuring the electrocatalytic signal generated ; ( d ) contacting the immobilized probe to a solution containing : ( i ) a sample thought to include the target nucleic acid , and ( ii ) a transition metal complex ; ( e ) measuring the electrocatalytic signal generated ; wherein an increase in the signal detected in step ( e ) over the signal generated in step ( c ) indicates that hybridization between the nucleic acid probe and the target nucleic acid has occurred . preferably , the transition metal of the transition metal complex is one selected from the group consisting of cobalt , iron , molybdenum , osmium , ruthenium and rhenium . more preferably , the transition metal of the transition metal complex is ruthenium . also preferably , the transition metal complex is a transition metal ammonium complex . more preferably , the first transition metal ammonium complex comprises a transition metal selected from the group consisting of cobalt , iron , molybdenum , osmium , ruthenium and rhenium . most preferably , the transition metal ammonium complex is ru ( nh 3 ) 6 3 + . the solutions can also include a second transition metal complex to enhance the electrocatalytic signal generated . preferably , the transition metal of the second transition metal complex is one selected from the group consisting of cobalt , molybdenum , osmium and rhenium . more preferably , the transition metal of the second transition metal complex is iron . also preferably , the second transition metal complex is a transition metal cynate complex . more preferably , the second transition metal cynate complex comprises a transition metal selected from the group consisting of cobalt , molybdenum , osmium and rhenium . most preferably , the second transition metal cynate complex is fe ( cn ) 6 − 3 . the method can also include rinsing steps , e . g ., rinsing the electrode between contact with the different solutions . another aspect of the invention additionally features a method of detecting the presence of a target nucleic acid in a sample , wherein the method includes the following steps : ( a ) providing a nucleic acid probe immobilized on a solid support ; ( b ) contacting the immobilized probe to a solution containing : ( i ) a transition metal complex ; ( c ) measuring the electrocatalytic signal generated ; ( d ) contacting the immobilized probe to a solution containing : ( i ) a sample thought to include the target nucleic acid , and ( ii ) a transition metal complex ; ( e ) measuring the electrocatalytic signal generated ; wherein an increase in the signal detected in step ( e ) over the signal generated in step ( c ) indicates the target nucleic acid is present in the sample . preferably , the transition metal of the transition metal complex is one selected from the group consisting of cobalt , iron , molybdenum , osmium , ruthenium and rhenium . more preferably , the transition metal of the transition metal complex is ruthenium . also preferably , the transition metal complex is a transition metal ammonium complex . more preferably , the first transition metal ammonium complex comprises a transition metal selected from the group consisting of cobalt , iron , molybdenum , osmium , ruthenium and rhenium . most preferably , the transition metal ammonium complex is ru ( nh 3 ) 6 3 + . the solutions can also include a second transition metal complex to enhance the electrocatalytic signal generated . preferably , the transition metal of the second transition metal complex is one selected from the group consisting of cobalt , molybdenum , osmium and rhenium . more preferably , the transition metal of the second transition metal complex is iron . also preferably , the second transition metal complex is a transition metal cynate complex . more preferably , the second transition metal cynate complex comprises a transition metal selected from the group consisting of cobalt , molybdenum , osmium and rhenium . most preferably , the second transition metal cynate complex is fe ( cn ) 6 − 3 . the method can also include rinsing steps , e . g ., rinsing the electrode between contact with the different solutions . the invention further features a method of detecting a mismatch between two nucleic acids , where the method includes the following steps : ( a ) providing a nucleic acid probe immobilized on a solid support ; ( b ) contacting the immobilized probe to a solution containing : ( i ) a transition metal complex ; ( c ) measuring the electrocatalytic signal generated ; ( d ) contacting the immobilized probe to a solution containing : ( i ) a sample thought to include the target nucleic acid , and ( ii ) a transition metal complex ; ( e ) measuring the electrocatalytic signal generated ; wherein a decrease in the signal detected in step ( e ) over the signal generated in step ( c ) indicates that there is a mismatch between the nucleic acid probe and the target nucleic acid . preferably , the transition metal of the transition metal complex is one selected from the group consisting of cobalt , iron , molybdenum , osmium , ruthenium and rhenium . more preferably , the transition metal of the transition metal complex is ruthenium . also preferably , the transition metal complex is a transition metal ammonium complex . more preferably , the first transition metal ammonium complex comprises a transition metal selected from the group consisting of cobalt , iron , molybdenum , osmium , ruthenium and rhenium . most preferably , the transition metal ammonium complex is ru ( nh 3 ) 6 3 + . the solutions can also include a second transition metal complex to enhance the electrocatalytic signal generated . preferably , the transition metal of the second transition metal complex is one selected from the group consisting of cobalt , molybdenum , osmium and rhenium . more preferably , the transition metal of the second transition metal complex is iron . also preferably , the second transition metal complex is a transition metal cynate complex . more preferably , the second transition metal cynate complex comprises a transition metal selected from the group consisting of cobalt , molybdenum , osmium and rhenium . most preferably , the second transition metal cynate complex is fe ( cn ) 6 − 3 . the method can also include rinsing steps , e . g ., rinsing the electrode between contact with the different solutions . in any of the methods described herein , the solid support can be a gold electrode . the target nucleic acid that is detected by the method of the present invention can be , for example , single - stranded or double - stranded dna , single - stranded or double - stranded rna , or a hybrid of dna and rna . the target also can be a polynucleotide , e . g ., in a purified or non - purified form . the sample of nucleic acids can be drawn from any source and can be natural or synthetic . the sample of nucleic acid may contain of deoxyribonucleic acids ( dna ), ribonucleic acids ( rna ), or copolymers of deoxyribonucleic acid and ribonucleic acid or combinations thereof . the target polynucleotide can be synthesized enzymatically or chemically in vitro , or be synthesized non - enzymatically . the sample containing the target polynucleotide can also comprise extragenomic dna from an organism , rna transcripts thereof , or cdna prepared from rna transcripts thereof . also , the target polynucleotide can be synthesized by the polymerase or ligase chain reaction . preferably , the nucleic acid probe is a sequence that is known to be unique to the target nucleic acid ( e . g ., pathogen ) being detected . such unique sequences are known for a number of pathogens , and methods for obtaining such unique sequences are also known ( see , e . g ., u . s . pat . no . 4 , 900 , 659 , “ nucleotide sequence composition and method for detection of neisseria gonorrhoeae and method for screening for a nucleotide sequence that is specific for a genetically distinct group ”). the probe sequence is capable of binding to the target nucleic acid of complementary sequence through one or more types of chemical bonds including base pairing . among the target nucleic acid which can be detected using the molecular probe of the invention is genetic material in the form of dna or rna obtained from any naturally occurring prokaryotes such as for example , pathogenic or non - pathogenic bacteria including but not limited to species of escherichia , salmonella , clostridium , chlamydia , etc ., eukaryotes such as for example , protozoans and parasites , fungi , yeast , higher plants , insects , lower and higher animals , including mammals and humans and cells in tissue culture , or viruses such as for example , herpes viruses , hiv , influenza virus , epstein - barr virus , hepatitis b virus , etc . target nucleic acids from these sources may , for example , be found in samples of a bodily fluid from an animal , including a human , such as , but not limited to , blood , urine , lymphatic fluid , synovial fluid , bile , phlegm , saliva , menstrual fluid and semen . in addition , samples containing dna or rna may , for example , be found in fluids from a plant , such as , but not limited to , xylem fluid , phloem fluid and plant exudates . samples containing dna or rna may , for example also be found in non - living sources such as , but not limited to , food , sewage , forensic samples , lakes , reservoirs , rivers and oceans . target polynucleotides can also be those of defunct or extinct organisms , e . g ., pressed plants in herbarium collections , or from pelts , taxidermy displays , fossils , or those of biological materials in museum collections . the target nucleic acid molecule may optionally be amplified prior to detection by the method of the present invention . the target nucleic acid can be in either a double - stranded or single - stranded form . in the case where the target nucleic acid molecule is double - stranded , it is preferably first treated by a denaturation agent to render the two strands into a single - stranded , or partially single - stranded form , at the start of the amplification reaction , by methods known in the art such as heating , alkali treatment , or by enzymatic methods . general methods for accomplishing this treatment are provided by sambrook , j . et al ., molecular cloning : a laboratory manual , cold spring harbor laboratory press , cold spring harbor , n . y ., u . s . a . ( 1989 ). once the sample has been treated to expose any target nucleic acid , the solution can be tested as described herein to detect hybridization between the attached nucleic acid and the target nucleic acid , if such is present . alternatively , some samples can be tested directly , e . g ., the target may exist in a serum sample and can be directly accessible , and may not require treatment to release the nucleic acid . a nucleic acid molecule is “ hybridizable ” to another nucleic acid molecule , such as a cdna , genomic dna , or rna , when a single stranded form of the nucleic acid molecule can anneal to the other nucleic acid molecule under the appropriate conditions of temperature and solution ionic strength ( see sambrook et al ., molecular cloning : a laboratory manual , cold spring harbor laboratory press ). the conditions of temperature and ionic strength determine the “ stringency ” of the hybridization . for preliminary screening for homologous nucleic acids , low stringency hybridization conditions , corresponding to a t m of 55 ° c ., can be used , e . g ., 5 × ssc , 0 . 1 % sds , 0 . 25 % milk , and no formamide ; or 30 % formamide , 5 × ssc , 0 . 5 % sds ). moderate stringency hybridization conditions correspond to a higher t m , e . g ., 40 % formamide , with 5 × or 6 × scc . high stringency hybridization conditions correspond to the highest t m , e . g ., 50 % formamide , 5 × or 6 × scc . hybridization requires that the two nucleic acids contain complementary sequences , although depending on the stringency of the hybridization , mismatches between bases are possible . the appropriate stringency for hybridizing nucleic acids depends on the length of the nucleic acids and the degree of complementary , variables well known in the art . the greater the degree of similarity or homology between two nucleotide sequences , the greater the value of t m for hybrids of nucleic acids having those sequences . the relative stability ( corresponding to higher t m ) of nucleic acid hybridizations decreases in the following order : rna : rna , dna : rna , dna : dna . for hybrids of greater than 100 nucleotides in length , equations for calculating t m have been derived ( see sambrook et al ., supra , 9 . 50 - 0 . 51 ). for hybridization with shorter nucleic acids , i . e ., oligonucleotides , the position of mismatches becomes more important , and the length of the oligonucleotide determines its specificity ( see sambrook et al ., supra , 11 . 7 - 11 . 8 ). preferably a minimum length for a hybridizable nucleic acid is at least about 10 nucleotides ; preferably at least about 15 nucleotides ; and more preferably the length is at least about 20 nucleotides ; and most preferably 30 nucleotides . “ high stringency hybridization conditions ” can employ hybridization at either ( 1 ) 1 × ssc ( 10 × ssc = 3 m nacl , 0 . 3 m na 3 - citrate . 2h 2 o ( 88 g / liter ), ph to 7 . 0 with 1 m hcl ), 1 % sds ( sodium dodecyl sulfate ), 0 . 1 - 2 mg / ml denatured salmon sperm dna at 65 ° c ., ( 2 ) 1 × ssc , 50 % formamide , 1 % sds , 0 . 1 - 2 mg / ml denatured salmon sperm dna at 42 ° c ., ( 3 ) 1 % bovine serum albumen ( fraction v ), 1 mm na 2 . edta , 0 . 5 m nahpo 4 ( ph 7 . 2 ) ( 1 m nahpo 4 = 134 g na 2 hpo 4 . 7h 2 o , 4 ml 85 % h 3 po 4 per liter ), 7 % sds , 0 . 1 - 2 mg / ml denatured salmon sperm dna at 65 ° c ., ( 4 ) 50 % formamide , 5 × ssc , 0 . 02 m tris - hcl ( ph 7 . 6 ), 1 × denhardt &# 39 ; s solution ( 100 ×= 10 g ficoll 400 , 10 g polyvinylpyrrolidone , 10 g bovine serum albumin ( fraction v ), water to 500 ml ), 10 % dextran sulfate , 1 % sds , 0 . 1 - 2 mg / ml denatured salmon sperm dna at 42 ° c ., ( 5 ) 5 × ssc , 5 × denhardt &# 39 ; s solution , 1 % sds , 100 g / ml denatured salmon sperm dna at 65 ° c ., or ( 6 ) 5 × ssc , 5 × denhardt &# 39 ; s solution , 50 % formamide , 1 % sds , 100 μg / ml denatured salmon sperm dna at 42 ° c ., with high stringency washes of either ( 1 ) 0 . 3 - 0 . 1 × ssc , 0 . 1 % sds at 65 ° c ., or ( 2 ) 1 mm na 2 edta , 40 mm nahpo 4 ( ph 7 . 2 ), 1 % sds at 65 ° c . the above conditions are intended to be used for dna - dna hybrids of 50 base pairs or longer . where the hybrid is believed to be less than 18 base pairs in length , the hybridization and wash temperatures should be 5 - 10 ° c . below that of the calculated t m of the hybrid , where t m in ° c .=( 2 × the number of a and t bases )+( 4 × the number of g and c bases ). for hybrids believed to be about 18 to about 49 base pairs in length , the t m in ° c .=( 81 . 5 ° c .+ 16 . 6 ( log 10 m )+ 0 . 41 (% g + c )− 0 . 61 (% formamide )− 500 / l ), where “ m ” is the molarity of monovalent cations ( e . g ., na + ), and “ l ” is the length of the hybrid in base pairs . “ moderate stringency hybridization conditions ” can employ hybridization at either ( 1 ) 4 × ssc , ( 10 × ssc = 3 m nacl , 0 . 3 m na 3 - citrate . 2h 2 o ( 88 g / liter ), ph to 7 . 0 with 1 m hcl ), 1 % sds ( sodium dodecyl sulfate ), 0 . 1 - 2 mg / ml denatured salmon sperm dna at 65 ° c ., ( 2 ) 4 × ssc , 50 % formamide , 1 % sds , 0 . 1 - 2 mg / ml denatured salmon sperm dna at 42 ° c ., ( 3 ) 1 % bovine serum albumen ( fraction v ), 1 mm na 2 . edta , 0 . 5 m nahpo 4 ( ph 7 . 2 ) ( 1 m nahpo 4 = 134 g na 2 hpo 4 . 7h 2 o , 4 ml 85 % h 3 po 4 per liter ), 7 % sds , 0 . 1 - 2 mg / ml denatured salmon sperm dna at 65 ° c ., ( 4 ) 50 % formamide , 5 × ssc , 0 . 02 m tris - hcl ( ph 7 . 6 ), 1 × denhardt &# 39 ; s solution ( 100 ×= 10 g ficoll 400 , 10 g polyvinylpyrrolidone , 10 g bovine serum albumin ( fraction v ), water to 500 ml ), 10 % dextran sulfate , 1 % sds , 0 . 1 - 2 mg / ml denatured salmon sperm dna at 42 ° c ., ( 5 ) 5 × ssc , 5 × denhardt &# 39 ; s solution , 1 % sds , 100 μg / ml denatured salmon sperm dna at 65 ° c ., or ( 6 ) 5 × ssc , 5 × denhardt &# 39 ; s solution , 50 % formamide , 1 % sds , 100 μg / ml denatured salmon sperm dna at 42 ° c ., with moderate stringency washes of 1 × ssc , 0 . 1 % sds at 65 ° c . the above conditions are intended to be used for dna - dna hybrids of 50 base pairs or longer . where the hybrid is believed to be less than 18 base pairs in length , the hybridization and wash temperatures should be 5 - 10 ° c . below that of the calclated t m of the hybrid , where t m in ° c .=( 2 × the number of a and t bases )+( 4 × the number of g and c bases ). for hybrids believed to be about 18 to about 49 base pairs in length , the t m in ° c .=( 81 . 5 ° c .+ 16 . 6 ( log 10 m )+ 0 . 41 (% g + c )− 0 . 61 (% formamide )− 500 / l ), where “ m ” is the molarity of monovalent cations ( e . g ., na + ), and “ l ” is the length of the hybrid in base pairs . “ low stringency hybridization conditions ” can employ hybridization at either ( 1 ) 4 × ssc , ( 10 × ssc = 3 m nacl , 0 . 3 m na 3 - citrate . 2h 2 o ( 88 g / liter ), ph to 7 . 0 with 1 m hcl ), 1 % sds ( sodium dodecyl sulfate ), 0 . 1 - 2 mg / ml denatured salmon sperm dna at 50 ° c ., ( 2 ) 6 × ssc , 50 % formamide , 1 % sds , 0 . 1 - 2 mg / ml denatured salmon sperm dna at 40 ° c ., ( 3 ) 1 % bovine serum albumen ( fraction v ), 1 mm na 2 . edta , 0 . 5 m nahpo 4 ( ph 7 . 2 ) ( 1 m nahpo 4 = 134 g na 2 hpo 4 . 7h 2 o , 4 ml 85 % h 3 po 4 per liter ), 7 % sds , 0 . 1 - 2 mg / ml denatured salmon sperm dna at 50 ° c ., ( 4 ) 50 % formamide , 5 × ssc , 0 . 02 m tris - hcl ( ph 7 . 6 ), 1 × denhardt &# 39 ; s solution ( 100 ×= 10 g ficoll 400 , 10 g polyvinylpyrrolidone , 10 g bovine serum albumin ( fraction v ), water to 500 ml ), 10 % dextran sulfate , 1 % sds , 0 . 1 - 2 mg / ml denatured salmon sperm dna at 40 ° c ., ( 5 ) 5 × ssc , 5 × denhardt &# 39 ; s solution , 1 % sds , 100 μg / ml denatured salmon sperm dna at 50 ° c ., or ( 6 ) 5 × ssc , 5 × denhardt &# 39 ; s solution , 50 % formamide , 1 % sds , 100 μg / ml denatured salmon sperm dna at 40 ° c ., with low stringency washes of either 2 × ssc , 0 . 1 % sds at 50 ° c ., or ( 2 ) 0 . 5 % bovine serum albumin ( fraction v ), 1 mm na 2 edta , 40 mm nahpo 4 ( ph 7 . 2 ), 5 % sds . the above conditions are intended to be used for dna - dna hybrids of 50 base pairs or longer . where the hybrid is believed to be less than 18 base pairs in length , the hybridization and wash temperatures should be 5 - 10 ° c . below that of the calculated t m of the hybrid , where t m in ° c .=( 2 × the number of a and t bases )+( 4 × the number of g and c bases ). for hybrids believed to be about 18 to about 49 base pairs in length , the t m in ° c .=( 81 . 5 ° c .+ 16 . 6 ( log 10 m )+ 0 . 41 (% g + c )− 0 . 61 (% formamide )− 500 / l ), where “ m ” is the molarity of monovalent cations ( e . g ., na + ), and “ l ” is the length of the hybrid in base pairs . the assays described herein can be used to detect pathogens , such as bacteria or viruses , or can be used to detect the expression of genes in a subject . for instance , genes from helicobacter pylori , a pathogen implicated in gastric ulcers and cancer , were detected by the methods described herein . two sequences belonging to the pathogenic microbe helicobacter pylori are used to demonstrate the versatility and specificity of the assay : one that codes for an unique h . pylori protein and one that represents a small portion of the 23s rrna from this organism . both sequences can be detected into the nanomolar concentration range . in addition to reporting the presence of pathogen - related sequences , this assay can accurately resolve single - base changes in target sequences . an a2143c substitution within the h . pylori rrna that confers antibiotic resistance significantly attenuates hybridization to an immobilized probe corresponding to the wt sequence . the single base mismatch introduced by this mutation slows the kinetics of hybridization and permits discrimination of the two sequences at short hybridization times . the assay described may therefore provide a means to detect and genotype infectious bacteria using electrochemical methods . fig1 shows a schematic of the electrocatalytic dna hybridization detection system of the invention , which uses the increased loading of ru ( nh 3 ) 6 3 + resulting from the formation of a dna duplex to report hybridization . the introduction of fe ( cn ) 6 3 − makes the electrochemical reduction of this cation catalytic and amplifies the signal dramatically . fig2 illustrates representative data obtained using this approach to detect a synthetic 30 - mer modeling the hpn gene from helicobactor pylori , an infectious bacterium that is strongly linked with gastric ulcers and cancer . gold electrodes were modified with single - stranded probe sequence , the electrodes treated with mercaptohexanol , and incubated in two heated buffer solutions ( one which contained the target sequence ( fig2 a ), and the other which did not ( fig2 b ). hybridization conditions were 40 ° c ., 35 mm sodium phosphate , 100 mm nacl , 25 minutes , with or without 4 μm hpn target sequence : ( seq id no : 1 ) 5 ′- tgt tgc agc act agc gat agt cat cat caa - 3 ′ the electrode exposed to the target sequence exhibited a pronounced increase in the electrochemical response , while that incubated in a buffer solution displayed a decreased response ( this is a reproducible event — it appears that the heat treatment dislodges some loosely bound probe dna ). fig3 shows the excellent reproducibility of the assay . the invention is further illustrated by the following examples , which are not intended to be limiting . chemicals and materials . dna synthesis reagents were obtained from glen research . 1 , 6 - hexamethylenediamine , 99 . 8 % anhydrous 1 , 4 - dioxane , 6 - mercapto - 1 - hexanol ( 97 %) ( mch ), and potassium ferrocyanide trihydrate were received from aldrich chemical company . potassium ferricyanide , 1 , 1 ′- carbonyldiimidizole , and hexaammineruthenium chloride were purchased from acros organics . n - succinimidyl 3 -( 2 - pyridyldithio ) propionate ( spdp ) was purchased from pierce . dithiothreitol ( dtt ) and 2 - mercaptoethanol were obtained from fisher scientific . gold - coated silicon wafers were received from platypus technologies . cloned pfu dna polymerase was obtained from stratagene . preparation and purification of modified oligonucleotides . oligonucleotides were synthesized using an abi 394 dna / rna synthesizer according to standard automated solid - phase techniques . oligonucleotides modified at the 5 ′- terminus with hexanediamine - based linker ( c6 ) were prepared and purified as described previously . 25 all unmodified oligonucleotides were stringently purified using reversed phase hplc . the following probe and target sequences were used in experiments employing synthetic oligonucleotides : hp1a ( 30 nt complementary hpn probe ): ( seq id no : 12 ) sh - 5 ′ ttgatgatgactatcgctagtgctgcaaca 3 ′ hp1b ( 18 nt + 12t complementary hpn probe ) ( seq id no : 4 ) sh - 5 ′ ttttttttttttgatgactatcgctagtgc 3 ′ hp1c ( 18 nt + 12t noncomplementary hpn probe ) ( seq id no : 5 ) sh - 5 ′ ttttttttttttgggataattcttcaccgg 3 ′ hp2a ( rrna probe ): ( seq id no : 13 ) sh - 5 ′ gggtctttccgtcttgcc 3 ′ hp2b ( rrna probe - 2 ): ( seq id no : 14 ) sh - 5 ′ ggtccacggggtctttcc 3 ′ t1 ( hpn target ) ( seq id no : 1 ) 5 ′ tgttgcagcactagcgatagtcatcatcaa 3 ′ t2a ( wt rrna target ): ( seq id no : 2 ) 5 ′ ggcaagacggaaagaccc 3 ′ t2amut ( a2143c rrna target ): ( seq id no : 3 ) 5 ′ ggcaagacgga c agaccc 3 ′ t2b ( wt rrna target # 2 ): ( seq id no : 15 ) 5 ′ ggaaagaccccgtggacc 3 ′ t2bmut ( a2143c rrna target # 2 ): ( seq id no : 16 ) 5 ′ gga c agaccccgtggacc 3 ′ ( in both a2143c rrna sequences , the site of the resistance mutation is underlined .) t - nc ( noncomplementary target ): ( seq id no : 17 ) 5 ′ aac agt tcc tgc atg 3 ′ probe strands featuring fluoresecein attached to the base at the 3 ′- terminus were synthesized using a fluorescein - dt cpg ( glen research ) and modified with a thiol - terminated linker as described previously . fluorescein attachment to target strands was achieved with a 5 ′- fluorescein phosphoramidite following standard automated solid phase techniques . fluorescein - modified oligonucleotides were purified by reversed phase hplc . modification of gold surfaces with probe dna . single - stranded thiolated probes were immobilized on bulk gold electrodes with a = 0 . 02 cm 2 ( bioanalytical systems ). prior to probe immobilization , gold electrodes were polished using 0 . 05 μm alumina , rinsed in water , sonicated for 5 mm , etched by scanning from 0 - 1 . 8 v at 200 mv / sec in 1m h 2 so 4 , and rinsed with water . inverted gold electrodes were typically exposed to ssdna thiolated probes in solutions containing 5 μm sh - dna , 500 nm mch , 25 mm sodium phosphate ( ph 7 ), 25 mm nacl , and 50 mm mgcl 2 in a humidity chamber at room temperature for 1 hour . ( any deviations from these conditions are described in individual figure captions .) manipulation of probe film densities was achieved with solutions containing variable amounts of mgcl 2 ranging from 10 - 100 mm . following deposition , electrodes were rinsed in 25 mm sodium phosphate ( ph 7 ), 25 mm nacl buffer . the adsorption of dna on the electrode surface was confirmed by monitoring the blocking of 2 mm ferrocyanide in 25 mm sodium phosphate ( ph 7 ), 25 mm nacl . hybridization of target sequences . gold electrodes modified with thiolated ssdna were exposed to target sequences and hybridization was detected through enhancement of the electrocatalytic signal . prior to hybridization of target , initial electrocatalytic measurements of immobilized ssdna probes were recorded and upon hybridization of target the change in signal could be calculated . electrochemical measurements . electrochemical measurements were conducted with a bioanalytical systems cv - 50 potentiostat . a one - compartment cell fitted with a luggin capillary was used . all cyclic voltammetry measurements were conducted at room temperature with a bioanalytical systems cv - 50w potentiostat . a three - electrode configuration was used consisting of a modified gold working electrode , a platinum wire auxiliary electrode , and an ag / agcl reference electrode . a one - compartment cell fitted with a luggin capillary was used to separate the working compartment from the reference compartment . electrocatalytic currents were measured in solutions of 2 mm fe ( cn ) 6 3 − , 27 μm ru ( nh 3 ) 6 3 + in 25 mm sodium phosphate / 250 mm nacl ( ph 7 ) at a scan rate of 100 mv / s . cathodic charge ( q ) was quantitated by integrating background - subtracted voltammograms . signal changes corresponding to hybridization were calculated as follows δq =( q final − q initial )/ q initiail . error bars shown on individual figures correspond to variabilities among multiple independent trials of each experiment . the electrocatalytic current obtained at gold electrodes modified with thiolated probe dna was measured , and rinsed electrodes were then exposed to target sequences and hybridization was detected through enhancement of the electrocatalytic signal . hybridization solutions typically contained 500 nm - 20 μm target dna in 25 mm sodium phosphate ( ph 7 ), 25 mm nacl , 100 mm mgcl 2 . electrodes were incubated at 37 - 50 ° c . in a thermostatted humidity chamber and were washed extensively with buffer before electrochemical analysis . the conditions used for individual experiments varied depending on the size and source of the target nucleic acid ; details of different hybridization trials are provided in the figure captions . quanatitation of electrode surface coverage using fluorescein - labeled dna was achieved based on the procedure described by demers et al . prior to the deposition of fluorophore - labeled dna , bulk gold electrodes were prepared as described above with electrochemical etching . larger ( 0 . 28 cm 2 ) flat gold surfaces were cleaned in piranha solution ( 3 : 1h 2 so 4 / h 2 o 2 ) for 20 minutes followed by stringent washing in water . using a guide producing an area of 0 . 28 cm 2 , 3 ′- fluorescein - 5 ′- thiol modified oligonucleotide was incubated on the gold surface for 1 hour at room temperature in a humidity chamber . probe immobilization was performed using a solution containing 5 μm 3 ′- fluorescein - 5 ′- thiol probe , 500 nm mch , 25 mm sodium phosphate ( ph 7 ), 25 mm nacl and varied amounts of mgcl 2 ( 10 mm to 100 mm ). substrates treated with noncomplementary probes were used as controls . after deposition , gold surfaces were washed extensively with 25 mm sodium phosphate ( ph 7 ), 25 mm nacl . fluorophore - modified probes were then displaced with 12 mm mercaptoethanol for approximately 3 - 4 hours at room temperature in a humidity chamber ; a second round of displacement was conducted overnight . fluorescence intensities for calibration standards and samples removed from the gold surface were measured in 50 mm naoh ( ph 12 ) on a wallac victorf fluorescence plate reader . amounts of 3 ′- fluorescein - 5 ′- thiol modified oligonucleotide displaced from the surface were determined by interpolation from a standard linear calibration curve prepared with known concentrations of the modified probe . for the measurement of hybridization efficiencies using fluorescence , labeled target sequences were introduced from solutions containing 5 μm target ( f1 - t2 ), 25 mm sodium phosphate ( ph 7 ), 25 mm nacl , and 100 mm mgcl 2 for 1 hour in a 40 ° c . incubator . the surfaces were then stringently washed with 25 mm sodium phosphate ( ph 7 ), 25 mm nacl to remove non - hybridized target . displacement of duplexes and fluorescence measurements were performed as described above . a standard linear calibration curve was plotted using known concentrations of duplex dna ( hp2a / f1 - t2 ). thermal denaturation measurements were performed with solutions containing 1 μm of complementary strands in 25 mm sodium phosphate ( ph 7 ), 25 mm nacl . measurements were obtained by monitoring absorbance at 260 nm on an aviv spectrophotometer . the appendage of a thiol - terminated linker to synthetic oligonucleotides permits the self - assembly of dna films on gold electrodes . gold surfaces modified with single - stranded oligonucleotides have been prepared by several groups interested in monitoring electrochemical processes in the presence of dna . the films used in the experiments described here feature oligonucleotides containing an aliphatic linker that is attached post - synthetically using a combination of solid - and solution - phase synthesis . a co - adsorbent , mercaptohexanol , is introduced during deposition to decrease the density of adsorbed dna and to minimize non - specific dna binding at the gold surface . the conditions employed here for deposition produce high - density films from thiol - modified oligonucelotides within minutes and have coverages that depend on the amount of divalent cation used in the deposition solution . using fluorescein - modified oligonucleotides , it was determined that densities of 12 (± 2 ), 23 (± 3 ), and 27 (± 4 ) pmol / cm 2 of single - stranded oligonucleotides were obtained with 10 , 50 , or 100 mm mgcl 2 present in the deposition buffer , respectively . probe - density measurements were made both on bulk gold electrodes and vapor - deposited gold substrates to confirm that comparable densities existed ( working with the larger substrates was desirable for more accurate quantitation of the less dense coverages ). coverages comparable to those measured here with low [ mg 2 + ] were observed in previous studies where deposition was performed in the presence of 10 mm sodium phosphate and 100 mm nacl . for the electrochemical experiments described below , dna films were used that were formed with 50 mm mgcl 2 present during deposition . while sparser surface coverages promote more efficient dna hybridization ( vide infra ), greater reproducibility was achieved with higher dna densities that produced larger voltammetric signals . detection of target dna sequences based on the electrocatalytic reduction of ru ( nh 3 ) 6 3 + at dna - modified surfaces ru ( nh 3 ) 6 3 + , lacking any ligands that can bind to dna intercalatively , associates electrostatically with the negatively charged backbone . it is therefore a sequence - neutral binder and an ideal probe for quantitating dna adsorbed on an electrode surface . 26 monitoring hybridization with ru ( nh 3 ) 6 3 + would potentially provide a means to detect dna electrochemically . however , the films with sparser surface coverages that permit efficient hybridization only yield small signals for this redox - active species . to amplify signals obtained at dna - modified electrodes in the presence of ru ( nh 3 ) 6 3 + , we introduced an oxidant , fe ( cn ) 6 3 − , that would permit turnover of ru ( nh 3 ) 6 3 + by regenerating the oxidized form ( fig4 ). as shown in fig5 , large , irreversible reductive waves are observed at dna - modified electrodes immersed in solutions of fe ( cn ) 6 3 − and ru ( nh 3 ) 6 3 + , consistent with the proposed reaction cycle ( fig5 ). the electrochemical signals obtained with dna - modified electrodes from solutions of ru ( iii ) and fe ( iii ) are amplified by ˜ 100 - fold over those obtained when only ru ( nh 3 ) 6 3 + is present ( no signal is obtained in this region when only fe ( cn ) 6 3 − is present ). the electrocatalysis requires dna to attract the cation to the gold surface , as no signal is observed with a bare electrode . this assay sensitively reports the presence of a target dna sequence . the ru ( iii )/ fe ( iii ) signal monitored at a gold electrode modified with a probe sequence complementary to a portion of the h . pylori 23s rrna gene ( sequence : 5 ′- ggc aag acg gaa aga ccc - 3 ′ ( seq id no : 2 )) significantly increases after exposure of the electrode to a synthetic target oligonucleotide ( fig5 ). the change in the electrochemical response is barely detectable in the absence of fe ( iii ). short hybridization times (& lt ; 1 hour ) under mild conditions ( 40 ° c .) are sufficient to observe an increase in the electrocatalytic signal of & gt ; 100 %. in the presence of noncomplementary sequences or buffer lacking any dna , no appreciable signal differences are observed . the ru ( iii )/ fe ( iii ) electrocatalysis accurately reports hybridization of sequences of difference lengths and base composition . both the 18 - nt 23s rrna sequence described above and a 30 - nt sequence corresponding to a fragment of the hpn gene ( which encodes a protein unique to h . pylori , sequence : 5 ′- tgt tgc agc act agc gat agt cat cat caa - 3 ′ ( seq id no : 1 )) can be detected as shown in fig5 a . it is also sensitive , as target concentrations down to 10 nm produced measurable increases in the electrochemical response after hybridization . in experiments monitoring the hybridization of dna oligonucleotides corresponding to a region of the h . pylori 23s rrna , a pronounced sensitivity to mismatched base pairs within the target / probe complex was observed . the enhancement in the electrochemical signal typically observed with the wt rrna sequence was significantly diminished when an a - to - c substitution at position 2143 within the 23s rrna was introduced ( sequence : 5 ′- ggc aag acg gac aga ccc - 3 ′ ( seq id no : 3 ), the nucleotide corresponding to c2143 is in lower case ). the a2143c variant is important because this substitution imparts resistance to clarithromycin , the antibiotic typically used to combat h . pylori , and about 10 % of the infections observed clinically are clarithromycin resistant . the discrimination of the a2143c mutant is a result of slower hybridization kinetics for the sequence that is mismatched with respect to the probe . a systematic study of the hybridization efficiency as a function of time for the wt versus a2143c target revealed that the extent of hybridization for the two sequences only becomes comparable with incubation times over 12 hours . the pronounced effect caused by the single - base mismatch within the target / probe complex is a significant finding . previous studies of duplex hybridization in solution by other groups have characterized much more subtle effects , with association rates for two dna oligonucleotides displaying little sensitivity to the loss of a single watson - crick pair , and dissociation rates that increase by about an order of magnitude in mismatched assemblies . 27 therefore , it appears that heterogeneous hybridization reactions , with one oligonucleotide immobilized on an electrode surface , are much more sensitive to mismatches , a finding that provides the basis for distinguishing similar sequences with an electrochemical hybridization assay . the probe density that we use in our experiments also appears to amplify the effect , as studies using surface plasmon resonance to follow hybridization at gold surfaces with very low surface coverages have elucidated similar , but much less pronounced , effects . 22 a surface with a high coverage of negatively charged oligonucleotides may serve to further destabilize mismatched target / probe duplexes . the electrocatalytic dna detection assay described provides a sensitive and specific means to execute electrochemical genotyping . the method described will be useful for genetic analysis in a multiplexed format . hpn target detection using pcr products , rna transcripts , and a synthetic 30 - mer two probe sequences were tested with the different targets : hp2a ( complementary hpn probe ) 5 ′- ttt ttt ttt ttt gat gac tat cgc tag tgc - 3 ′ ( seq id no : 4 ) and hp2b ( noncomplementary hpn probe ) 5 ′- ttt ttt ttt ttt ggg ata att ctt cac cgg - 3 ′ ( seq id no : 5 ). the appended thymine bases allowed for the probe to be more accessible to the target . the complementary probe effectively detects the presence of the different target nucleic acids using the elctrocatalytic ru ( iii )/ fe ( iii ) system . pcr ( generated using asymmetric pcr as single - stranded dna , portion complementary to probe is underlined ): ( seq id no : 6 ) 5 ′- gga gtc atc atg gca cac cat gaa gaa cag cac ggc ggt cat cac cac cat cac cac cac aca cac cac cac cac tat cac ggc ggt gaa cac cac cat cac cac cac agc tct cat cat gaa gaa ggt tgt tgc agc act agc gat agt cat cat c at caa gaa gag ggt tgc tgc cac ggg cat cac gag taa tat cgg tgt ggc tag ggg caa ctt - 3 ′ rna ( same sequence as pcr product , generated in vitro from dna template , portion complementary to probe is underlined ): ( seq id no : 7 ) 5 ′ atc aaa gga gtc atc atg gca cac cat gaa gaa cag cac ggc ggt cat cac cac cat cac cac cac aca cac cac cac cac tat cac ggc ggt gaa cac cac cat cac cac cac agc tct cat cat gaa gaa ggt tgt tgc a gc act agc gat agt cat cat cat caa gaa gag ggt tgc tgc cac ggg cat cac gag taa tat cgg tgt ggc tag ggg caa ctt - 3 ′ ( seq id no : 8 ) 5 ′- tgt tgc a gc act agc gat agt cat cat c at caa - 3 ′ dna probe solutions ( hp2a and hp2b ) containing 5 μm ssdna , 500 nm mch , 50 mm mgcl 2 , and 25 mm sodium phosphate / nacl buffer ph 7 were deposited for 1 . 5 hours at room temperature in humidity chamber . target solution containing synthetic 30 - mer and pcr product contained 500 nm target , 100 mm mgcl 2 , and 25 mm sodium phosphate / nacl buffer ph 7 and were exposed to dna films for 1 hour at 45 ° c . rna target hybridization was under the same conditions except 1 μm target was used . the results are shown in fig7 , which is a bar graph showing the time dependence of hybridization for hp2a probe ( complementary hpn probe ) and hp2b probe ( noncomplementary hpn probe ). it shows that target dna sequences can be detected as either pcr products or rna transcripts using the methods described herein . the h . pylori hpn gene was pcr amplified from a recombinant source ( an e . coli plasmid provided by dr . andrew plaut of tufts university ). two pcr products were generated , one using the asymmetric method that produces mainly single - stranded dna , and another using conventional pcr conditions that would generate a double - stranded product for t7 runoff transcription of rna . for the former reaction , a forward pcr primer ( 5 ′- atc aaa gga gtc atc atg gca cac - 3 ′ ( seq id no : 9 )) and reverse pcr primer ( 5 ′- aag ttg ccc cta gcc aca - 3 ′ ( seq id no : 10 )) were used in reactions containing 1 μg / ml of plasmid dna , 500 nm forward primer , 5 nm reverse primer , 1 × of cloned pfu dna polymerase reaction buffer ( 200 mm tris - hcl ( ph 8 . 8 ), 100 mm kcl , 100 mm ( nh 4 ) 2so4 , 20 mm mgso 4 , 1 % triton x - 100 , 1 mg / ml nuclease - free bovine serum albumin ), 1 mm dntps , and 2 . 5 u of cloned pfu dna polymerase , polymerase buffer and enzyme purchased from stratagene , in a total reaction volume of 100 μl . for the synthesis of the pcr product used for the generation of the rna transcript , a forward pcr primer containing the t7 polymerase promoter sequence ( 5 ′- gct agg taa tac gac tca cta tag gag tca tca tgg cac ac - 3 ′ ( seq id no : 11 )) was used with the same reaction conditions with the exception of the addition of 500 nm forward and 500 nm reverse primer . pcr was performed on a stratagene robocycler with 30 cycles at 94 ° c . for 2 minutes , 52 ° c . for 2 minutes , 72 ° c . for 3 minutes . pcr products were subjected to phenol - chloroform extraction and ethanol precipitation . rna target was transcribed from amplified dna template with t7 promoter region using standard conditions . the resultant dna and rna targets had the following sequences : 5 ′ ggagtcatcatggcacaccatgaagaacagcacggcggt ( seq id no : 6 ) catcaccaccatcaccaccacacacaccaccaccactatcacggcggtgaacacca ccatcaccaccacagctctcatcatgaagaaggttgttgca gcactagcgatagtca tcatc atcaagaagagggttgctgccacgggcatcacgagtaatatcggtgtggct aggggcaactt 3 ′ ( rna , 219 nt ) and 5 ′ atcaaaggagtcatcatggcacaccatgaagaacagcacggcggtcatcaccacc ( seq id no : 7 ) atcaccaccacacacaccaccaccactatcacggcggtgaacaccaccatcaccac cacagctctcatcatgaagaaggttgttgca gcactagcgatagtcatcat catcaa gaagagggttgctgccacgggcatcacgagtaatatcggtgtggctaggggcaact t 3 ′ ( dna , 225 nt ); the portion of the sequence that is complementary to the hp1b probe is underlined . electrocatalytic reduction of ru ( nh 3 ) 6 3 + at dna - modified surfaces ru ( nh 3 ) 6 3 + , lacking any ligands that can bind to dna intercalatively , associates electrostatically with the negatively charged backbone . it is therefore a sequence - neutral binder and an ideal probe for the quantitation of single - or double - stranded dna adsorbed on an electrode surface . however , the limited concentration of ru ( nh 3 ) 6 3 + localized at dna - modified electrodes yields a small current under conditions suitable for hybridization detection ( i . e . concentrations of ru ( iii ) sufficiently low to prohibit direct adsorption of the redox - active probe ). to provide maximal sensitivity for the detection of dna hybridization , we introduced an oxidant , fe ( cn ) 6 3 − , that would permit turnover of ru ( nh 3 ) 6 3 + by regenerating the oxidized form ( scheme 1 ), thereby significantly amplifying the response obtained . indeed , as shown in fig8 , large , irreversible reductive waves are observed using cyclic voltammetry ( cv ) at dna - modified electrodes immersed in solutions of fe ( cn ) 6 3 − and ru ( nh 3 ) 6 3 + , consistent with the proposed reaction . the amount of current observed reports the quantity of dna present at the electrode surface , as the response obtained at surfaces featuring different densities ( controlled by varying [ mg 2 + ] during deposition ) was directly dependent on the number of dna molecules immobilized . the electrochemical signals obtained with dna - modified electrodes from solutions of ru ( iii ) and fe ( iii ) are amplified by ˜ 100 - fold over those obtained when only ru ( nh 3 ) 6 3 + is present ( fig8 b inset ); no signal is obtained in this region when only fe ( cn ) 6 3 − is present ( data not shown ). the electrocatalysis requires dna to attract the cationic complex to the gold surface , as no signal is observed with a bare electrode . the electrocatalytic assay sensitively reports the presence of a complementary target dna sequence . the ru ( nh 3 ) 6 3 + / fe ( cn ) 6 3 − signal monitored at a gold electrode modified with a probe sequence complementary to a portion of the h . pylori 23s rrna gene ( nucleotides 2132 - 2149 ) significantly increases after exposure of the electrode to a synthetic target oligonucleotide ( fig8 b ). short hybridization times (& lt ; 1 hour ) and mild conditions are sufficient to observe an increase in the integrated charge of & gt ; 100 %. in the presence of noncomplementary sequences or buffer lacking any dna , no appreciable signal differences are observed . the ru ( iii )/ fe ( iii ) electrocatalysis accurately reports hybridization of sequences of different lengths . both the 18 nucleotide 23s rrna sequence described above and a 30 nucleotide sequence corresponding to a fragment of the hpn gene ( which encodes a histidine - rich protein of unknown function unique to h . pylori ) can be detected as shown in fig9 . thus , the assay described is versatile and is compatible with different probe sequence lengths and base composition . it is unnecessary to match the length of the target and probe , as experiments where the size of the target was increased by 10 - 15 nucleotides also produced successful hybridization detection ( data not shown ). the electrocatalytic assay is also sensitive , as target concentrations down to 10 nm ( 50 fmol ) produced measurable increases in the electrochemical response after hybridization . the efficiency of hybridization , investigated using the electrocatalytic assay and fluorescence - based quantitation , was sensitive to the density of the immobilized probe sequence ( fig1 ). as described above , the density of dna films prepared with different amounts of mgcl 2 present was monitored using fluorescein - modified oligonucleotides . as the amount of mg 2 + in the deposition solution increases , the density of probe increases , with films with 11 pmol dna / cm 2 obtained with 10 mm mgcl 2 and films with 27 pmol dna / cm 2 obtained with 100 mm mgcl 2 . the response obtained in the presence of ru ( nh 3 ) 6 3 + and fe ( cn ) 6 3 − was also monitored , and increased with the surface coverage . with the film prepared with 10 mm mgcl 2 , the average charge measured was 0 . 13 ( 5 ) μc , while with 100 mm mgcl 2 present during probe deposition , the average charge measured was 0 . 59 ( 5 ) μc . the correlation between these values and the density of probe dna indicates that the electrochemical signal exhibits a direct dependence on the concentration of immobilized dna present at the electrode surface . when signal increases upon hybridization were monitored for the electrodes with different surface coverages , it was observed that films with lower probe densities permitted more efficient target capture ( fig1 ). this effect has been observed in several studies and is proposed to arise because of steric crowding when local concentrations of immobilized dna are high . while the lowest density film studied here ( formed with 10 mm mgcl 2 ) allowed 87 (± 5 )% hybridization , the highest density film ( formed with 100 mm mgcl 2 ) displayed a much lower level of hybridization with 6 (± 2 )% efficiency . the films prepared with 50 mm mgcl 2 that were routinely used in the electrocatalysis assay also displayed only partial hybridization , with 7 (± 2 )% of probes forming a complex with a target dna sequence . it is noteworthy , however , that the electrocatalytic assay was able to resolve this low level of target complexation with a change in the integrated charge of typically & gt ; 100 %. based on the dimensions of duplex dna , ˜ 50 pmol / cm 2 is the maximal coverage of duplexes that can be achieved . therefore , it is apparent that the coverage of single - stranded probe must be well below this level to achieve efficient hybridization . in experiments monitoring the hybridization of dna oligonucleotides corresponding to a region of the h . pylori 23s rrna , a pronounced sensitivity to mismatched base pairs within the target / probe complex was observed . the enhancement in the electrochemical signal typically observed with the wt rrna sequence was significantly diminished when a sequence containing an a - to - c substitution at position 2143 was introduced ( fig9 ). the a2143c sequence is medically significant because this substitution imparts resistance to claritbromycin , the antibiotic typically used to combat h . pylori . over 10 % of the infections observed clinically are clarithromycin resistant . based on the thermal stabilities of the rrna sequences used for these experiments , the observation of differential hybridization is surprising . the target / probe duplexes formed from the ribosomal sequences employed for this study exhibited t m values of 58 ( 2 )° c . when fully matched , and 52 ( 2 )° c . when the a2143c mutation was present that produced a c - t mismatch . thus , it is reasonable to expect that both duplexes should be formed at the surface if the complexation was governed by thermodynamic stability . to investigate the origin of the differential hybridization observed in the presence of the point mutation , the time dependence of the hybridization was monitored ( fig1 ). with short incubation times , a pronounced difference in the signal obtained for the wt sequence was observed relative to the a2143c sequence . however , if the hybridization was permitted to proceed longer than 12 hours , comparable results were obtained with both sequences . therefore , the discrimination of the a2143c mutation is a result of slower hybridization kinetics for the sequence that is mismatched with respect to the probe . the rate of association for both sequences is likely similar , thus the observed change may reflect a faster dissociation rate for the mismatched complex that limits the accumulation of hybridized duplexes . the applicability of the electrocatalytic assay to the detection of large dna and rna targets was tested using a & gt ; 200 nucleotide sequence containing the h . pylori hpn gene ( fig1 ). for these hybridization experiments , probe sequences were employed containing a linker of 12 thymine residues that served to increase the accessibility of the portion of the oligonucleotide used for target capture . using mild hybridization conditions ( 1 hour , 45 ° c . ), single - 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