WO1998013520A1 - Dispositif et technique d'identification de sequence de nucleotides d'adn par spectroscopie laser - Google Patents

Dispositif et technique d'identification de sequence de nucleotides d'adn par spectroscopie laser Download PDF

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Publication number
WO1998013520A1
WO1998013520A1 PCT/EE1997/000003 EE9700003W WO9813520A1 WO 1998013520 A1 WO1998013520 A1 WO 1998013520A1 EE 9700003 W EE9700003 W EE 9700003W WO 9813520 A1 WO9813520 A1 WO 9813520A1
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Prior art keywords
nucleotides
dna
identification card
atoms
marker molecules
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PCT/EE1997/000003
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English (en)
Inventor
Karl Rebane
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University Of Tartu
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Publication date
Application filed by University Of Tartu filed Critical University Of Tartu
Priority to AU42961/97A priority Critical patent/AU4296197A/en
Publication of WO1998013520A1 publication Critical patent/WO1998013520A1/fr

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    • 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
    • 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 belongs to the field of molecular biology and laser spectroscopy, or , more specifically, to the field of identification of DNA primary structure by laser spectroscopic means.
  • the closest solution to the means proposed by the present invention appears to be a stream of liquid used in laser spectroscopy, in which DNA nucleotides are identified by detection at the single molecule level (SMD) (Peter M. Goodwin, Rhett L. Affleck,
  • the method closest to the one described in the present invention is the laser spectroscopy method referred to above, which consists of the following stages. First of all the nucleotides in the DNA molecule are marked with molecules emitting characteristic fluorescence spectra - the so-called markers - so as to make it possible to differentiate between one to four out of four nucleotides A,C,G, and T. Secondly, the nucleotides are separated in succession one by one, using for this purpose chemical methods or enzymes.
  • the separated nucleotides are, one by one, and in the order of separation transported into a thin, precisely oriented jet of liquid, making sure that the distance between adjacent nucleotides within the stream is big enough to allow excitation of each single nucleotide separately by means of a laser beam, thus evoking its characteristic fluorescence.
  • the other nucleotides are not subjected to excitation.
  • the nucleotides within the jet are identified and their sequence established via their markers' characteristic fluorescence at the level of single molecule detection (SMD). SMD will reveal, which nucleotide within the jet passed through the focus of the laser beam.
  • SMD single molecule detection
  • T - denotes the time within which the nucleotide passes through the laser beam' s focus
  • T 10 s.
  • the speed and efficiency of the method are lower, i.e. the number of nucleotides identified per second is smaller.
  • even slight ruffling of the surface of the stream of liquid may cause the marked nucleotides to miss the laser focus and some nucleotides to pass unnoticed.
  • a considerable shortcoming of the method used for measuring within the stream of liquid is the fact that the stream disappears immediately after the measurement, thus excluding the possibility of repeating the measurement procedure of the nucleotide sequence of the same DNA molecule, in order to verify the initial result.
  • the question is, how to guarantee high sensitivity and selectivity of spectroscopic detection, and make it possible to repeat the measurement procedure.
  • the present invention proposes a means and a method, which will guarantee high sensitivity and selectivity of spectroscopic detection and will allow the measuring procedure to be repeated.
  • the invention proposes a DNA identification card (IC)to be used, in which the sequence of nucleotides coincides with their sequence in DNA, and a method, in which the fluorescence spectra of the marker molecules or atoms carried on to the IC are measured by way of SMD or SMS.
  • IC DNA identification card
  • the aim of the present invention is to propose a means and a method for identification of nucleotide sequences within the DNA molecule by means of spectroscopy and high resolution laser spectroscopy, in which single nucleotides or groups of nucleotides which have been cut off from the end of a DNA molecule are transported by means of a jet of gas, or a continous stream of liquid, a stream composed of drops of liquid onto/into a solid surface in this way that the sequence of nucleotides remains identical with that within the DNA molecule, but the intermolecular distances between the adjacent nucleotides are larger than the wavelength of light by which the fluorescence of the marker molecules or atoms is exited.
  • the solid means is moved along a linear or spiral or some other trajectory against to the stream at a suitable speed (ca 1 cm /s ) .
  • a suitable speed ca 1 cm /s
  • the solid together with the nucleotides of fixed structure on/in it will form an identification card, which retains the sequence of nucleotides within the DNA molecule.
  • the IC will be the means for identifying the nucleotide sequence within DNA by laser spectroscopy.
  • the DNA nucleotides or their groups to be cut off the molecule are marked either before or after they are cut off the DNA molecule, or after they have been carried onto/into the surface of the IC by means of marker molecules or atoms having a characteristic spectra of fluorescence, and the nucleotides are identified and their sequence determined on/in the surface of the IC by laser optical SMD , either at room temperature or at lower temperatures .
  • the IC is cooled down to reach temperatures below 10 K and the nucleotides are identified on/in its surface by SMS of the solid's zero- phonon lines (ZPL), whereas the nucleotides or groups of nucleotides to be severed from the DNA molecule are marked with such marker-molecules or atoms which at temperatures below 10 K have in their fluorescence spectra an intense and narrow purely electronic zero-phonon line.
  • the advantage of the second embodiment of the method as compared to the prototype method of single molecule laser spectroscopic detection (SMD) in a jet of liquid, consists in that spectral selectivity of nucleotide sequence identification is raised by 4-5 orders of magnitude.
  • the drawings describe the intensity of fluorescence of the nucleotides, as dependent on the frequency of exitation, to illustrate the second version of the second embodiment.
  • the diameter of the circles denotes intensity of fluorescence of one single nucleotide at the given frequency of excitation ⁇ L1 (Fig. 1).
  • ⁇ L1 intensity of fluorescence of one single nucleotide at the given frequency of excitation ⁇ L1 (Fig. 1).
  • the frequency ⁇ L2 is closer to the peak value of ZPL than in case of ⁇ L ⁇ for nucleotides No 1 and 2, and farther for nucleotides No 3 and 4; ⁇ L2 happens to be at the beginning of the ZPL absorption contour for a new nucleotide No 5.
  • ⁇ L2 ⁇ Ll + ⁇ ; ⁇ ⁇ ⁇ ZPL
  • ⁇ ZPL the width of the zero-phonon line.
  • Fig. 3 at the frequency ⁇ 3 a different set of nucleotides gets excited, the frequency of excitation having been changed well over the ZPL width ⁇ Z L .
  • the present invention offers a means described below for determining the sequence of DNA nucleotides by laser spectroscopy.
  • the said means is a solid means onto/into which the nucleotides or their groups cut off from the DNA molecule are carried and where the nucleotides or their groups are placed from one another at distances exceeding the wavelength of light exciting the fluorescence of marker molecules or atoms, the nucleotides or their groups are marked before or after carrying with marker molecules or atoms forming the DNA identification card in which the nucleotide sequence corresponds to their sequence in DNA.
  • the fluorescence spectra of the marker molecules/atoms are measured on the solid means (DNA identification card) by the single molecule detection (SMD) or single impurity molecule spectroscopy (SMS) method.
  • SMD single molecule detection
  • SMS single impurity molecule spectroscopy
  • a plate or tape of polymer or paper can be used which is moved linearly or spirally or at some other suitable trajectory with respect to the liquid or gas stream at such speed (ca 1 cm s ⁇ ) that the nucleotides or their groups remain at distances exceeding the wavelength of light exciting the fluorescence of marker molecules or atoms.
  • the nucleotide sequence in the liquid or gas stream is transferred to the spatial nucleotide sequence onto/into the identification card while the distances between the nucleotides are bigger than the wavelength of light exciting the fluorescence of marker molecules or atoms. In such a way a fixed nucleotide structure is formed onto/into solid means which is called the identification card.
  • the DNA identification card is a solid means with nucleotides carried the onto/into it, the sequence of the nucleotides being identical with that of the DNA molecule and from which the fluorescence spectra of the marker molecules/atoms are measured by the single molecule detection (SMD) or single impurity molecule spectroscopy (SMS) method.
  • SMD single molecule detection
  • SMS single impurity molecule spectroscopy
  • the nucleotides or their groups cut off from the DNA molecule can be marked, additionally marked or re-marked on the identification card as well.
  • the second version of the second application described below is used which enables simultaneous detection of the nucleotide strip with width up to 10 _1 cm (cf. Fig. 1-3).
  • the DNA identification card obtained by appliction of the invention is a record file which can be repeatedly investigated from various aspects, and by using different methods, the results obtained in different laboratories can be measured again and compared. For example, it is possible to determine the higher-order correlations in the nucleotides location, to use coherent optical methods, among them holography of various kinds. It is possible to create data banks of natural samples of DNA molecules. Very high spectral resolution allows us to identify not only individual nucleotides, but also their n-membered sets where n can be tens. Therefore it is not indispensable that single nucleotides would be cut one by one.
  • the DNA identification card of a testee (patient) can be compared later, even years after, with the freshly prepared DNA identification card of the same tested organism.
  • the inconsiderable ageing of the identification card at low temperatures due to the diffusion and spectral diffusion can be compensated for very high precision of the above- mentioned SMS method.
  • the identification card can be measured and investigated at room temperatures, i.e. at ca 300 K by the SMD method similarly to the one described in the prototype method made in Prof. Keller's laboratory. At low temperatures (below 77 K) a better spectral resolution and identification card preservation is achieved.
  • the spectral selectivity increases 4-5 times in comparison with SMD method (detection in a stream of liquid without the identification card or at room temperature on the identification card) used in the prototype.
  • the difference and advantages are that using the identification card makes use of different methods and repeated measurements possible, also in different laboratories .
  • the method has two embodiments which consist of the following stages.
  • the first embodiment is the single molecule detection (SMD) on the level where spectral selectivity is not high.
  • SMD single molecule detection
  • the parts of the DNA molecule to be severed will be marked with marker molecules/atoms having characteristic fluorescence spectra either before or after they are cut off from DNA.
  • the same known markers are used, for example those which have been used at Prof. Keller's laboratory.
  • the nucleotides or their groups are cut off one by one from the end of the DNA molecule, for example by use of enzymes.
  • the cutting off and marking, incl . re-marking of the parts of the DNA molecule takes place at a suitable temperature, for example at room temperature. Higher temperature will essentially accelerate the cutting procedure - the temperature rise by 1° C will accelerate it up to 6 times .
  • the nucleotides or their groups which have been cut off are carried into the gas or liquid stream (drops) and transported with that onto/into the solid means (identification card).
  • identification card In the next stage of the method the nucleotides are identified and their sequence is established with laser optics by the SMD method and level.
  • the identification card measuring can occure at room temperature (300 K) or at lower temperatures. Spectral selectivity at room temperature is not high, therefore the variant where the identification card is cooled down to temperature below 77 K is used, which guarantees higher spectral selectivity and a better preservation of identification cards.
  • the other embodiment of the method based on the zero-phonon lines (ZPL) spectroscopy guarantees very high spectral selectivity when measuring on the identification card, and thanks to high-precision measurements of the spectra the reliability of results is increased essentially.
  • the difference from the first embodiment consists in the fact that the identification card is cooled down to 10 K and suitable markers with zero-phonon lines are selected.
  • the parts to be cut off from the DNA molecule are marked before or after they are cut off from the DNA with such marker molecules/atoms which at temperatures below 10 K have intense and narrow zero-phonon lines fluorescence spectra. Markers containing for example the ions of rare earth metals or organic molecules with porphyrine core are used as promoters of ZPL.
  • the nucleotides or their groups are cut off one by one from the end of the DNA molecule, using, for example, enzymes.
  • the severing and marking, incl. re-marking, of the parts of the DNA molecule takes place at a suitable temperature, for example at the room temperature.
  • the marking and re-marking can proceed either at room temperature or at higher or lower temperatures.
  • the peak value of the ZPL absorption cross- section increases at low temperatures considerably (up to 4- 5 orders of magnitude). Below 10 K thousands of impurity molecules and atoms are suitable for the present method, i.e.
  • the indicator of sensitivity and selectivity for spectroscopic detection - the absorption cross-section ⁇ o for ZPL - is for example at
  • the dye laser of a narrow (laser linewidth 1-2 Mhz) and stable frequency is used, for example Coherent Radiation Single Mode Dye Laser CR-699-29 which is pumped for example with an argon laser.
  • known systems with a photomultiplier as their base element are used (in this case FEV-79 whose quantum yield is up to 12% at the wavelength 633 nm); the signal is sampled with a multichannel analyzer (in the present case LP-4900). Additionally, measurement automation hard- and software were used.
  • the second embodiment of the present invention uses two versions of single impurity molecule spectroscopy (SMS) of solid state zero-phonon lines (ZPL) for exciting fluorescence of marked nucleotides.
  • SMS single impurity molecule spectroscopy
  • ZPL solid state zero-phonon lines
  • the nucleotide sequence can be identified not only along the one-dimensional line determined by a sharp laser focus (whith the focus diameter d within the range of 1 to 10 ⁇ ) whose width is d ; but also along a remarkably wider strip D, where D equals roughly from 100 to 1000 ⁇ m. Therefore the ruffling of the liquid stream will not interfere with the applicability of the present method.
  • the exciting light spot is sharply focused (i.e. reaching up to the diameter d which is close to the diffraction limit wavelength ⁇ , where d equals ⁇ or is a few times bigger).
  • This mode proves troublesome if the width of the nucleotides distribution strip r on the identification card is many times bigger than ⁇ and therefore renders necessary high precision scanning of one and the same section of spatial distribution many times (tens and hundreds of times).
  • excitation is performed by a nonsharply focused laser beam, where the focus diameter d exceeds the diffraction limit ⁇ tens or hundreds of times.
  • the nucleotides are identified within a 0.1-1 ram wide strip of the identification card by moving the identification card against the laser beam and one scan (or a few scans) along the stream track on the identification card is sufficient.
  • the precision of laser frequency scanning exceeds the ZPL width. Owing to the intensity dependence of fluorescence, microscopy will provide a frequency-and-space-domain view of all the marked nucleotides within the range approximately equal to D 2 (cf. Fig. 1-3).
  • the abovementioned second excitation mode is used in the case when D is approximately equal to 100 ⁇ m, but it is possible to achieve a tenfold, i.e. when D is approximately equal to 1 mm. Therefore the proposed SMS embodiment makes it possible to compensate for the identification card deviations from the given trajectory axis within the range of up to 1 mm by means of one spatial scan.
  • the presnt invention allows for spatial and spectral viewing and simultaneous very high spectral selectivity identification of lots of nucleotides or their groups located on the identification card within dimensions 0.01 -
  • the invention w ll both raise the speed of measuring and enhance its reliability.

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Abstract

La présente invention concerne un dispositif (carte ADN) et une technique permettant d'identifier la séquence de nucléotides d'ADN par spectroscopie laser. La carte ADN de l'invention est un support complet sur lequel s'appuient ou dans lequel se fixent, isolés de la molécule d'ADN, les nucléotides ou leurs groupes selon la même séquence que dans l'ADN, les nucléotides ou leurs groupes se plaçant en respectant entre eux des distances supérieures à la longueur d'ondes de la lumière provoquant la fluorescence de leurs molécules ou atomes marqueurs. L'identification des nucléotides ou de leurs groupes et la détermination de leurs séquences d'après la carte ADN utilisent le spectre de fluorescence des nucléotides marqués selon la technique de détection moléculaire simple (SMD) ou selon la technique de spectroscopie moléculaire simple (SMS). On obtient une résolution spectrale élevée en refroidissant la carte ADN à des températures inférieures à 10 °K et en utilisant des marqueurs spécifiques portant avec eux à ces températures dans les spectres d'excitation de la fluorescence des raies phonons nuls étroites et intenses.
PCT/EE1997/000003 1996-09-27 1997-09-26 Dispositif et technique d'identification de sequence de nucleotides d'adn par spectroscopie laser WO1998013520A1 (fr)

Priority Applications (1)

Application Number Priority Date Filing Date Title
AU42961/97A AU4296197A (en) 1996-09-27 1997-09-26 A means and a method for identification of the sequence of dna nucleotides by laser spectroscopy

Applications Claiming Priority (2)

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EE9600101A EE9600101A (et) 1996-09-27 1996-09-27 Vahend ja meetod DNA nukleotiidide järjestuse määramiseks laserspektroskoopia abil
EEP9600101 1996-09-27

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Cited By (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US9243284B2 (en) 2000-12-01 2016-01-26 Life Technologies Corporation Enzymatic nucleic acid synthesis: compositions and methods for inhibiting pyrophosphorolysis

Citations (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
WO1994018218A1 (fr) * 1993-02-01 1994-08-18 Seq, Ltd. Procedes et appareil de sequençage de l'adn
WO1996024689A1 (fr) * 1995-02-07 1996-08-15 Sargent Jeannine P Procede et appareil pour determiner la sequence de polynucleotides

Patent Citations (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
WO1994018218A1 (fr) * 1993-02-01 1994-08-18 Seq, Ltd. Procedes et appareil de sequençage de l'adn
WO1996024689A1 (fr) * 1995-02-07 1996-08-15 Sargent Jeannine P Procede et appareil pour determiner la sequence de polynucleotides

Non-Patent Citations (2)

* Cited by examiner, † Cited by third party
Title
DAVIS L M ET AL: "RAPID DNA SEQUENCING BASED UPON SINGLE MOLECULE DETECTION", GENETIC ANALYSIS TECHNIQUES AND APPLICATIONS, vol. 8, no. 1, 1991, pages 1 - 7, XP002039495 *
HARDING AND KELLER: "SINGLE-MOLECULE DETECTION AS AN APPROACH TO RAPID DNA SEQUENCING", TIBTECH, vol. 10, 1992, pages 55 - 57, XP002052227 *

Cited By (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US9243284B2 (en) 2000-12-01 2016-01-26 Life Technologies Corporation Enzymatic nucleic acid synthesis: compositions and methods for inhibiting pyrophosphorolysis

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EE9600101A (et) 1998-04-15

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