WO1993019358A1 - Fluorometer detection system - Google Patents

Fluorometer detection system Download PDF

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Publication number
WO1993019358A1
WO1993019358A1 PCT/US1993/002540 US9302540W WO9319358A1 WO 1993019358 A1 WO1993019358 A1 WO 1993019358A1 US 9302540 W US9302540 W US 9302540W WO 9319358 A1 WO9319358 A1 WO 9319358A1
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WO
WIPO (PCT)
Prior art keywords
time
fluorometer
laser diode
sample
laser
Prior art date
Application number
PCT/US1993/002540
Other languages
French (fr)
Inventor
Robert Marlin Studholme
David Arthur Blau
Original Assignee
Diatron Corporation
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Application filed by Diatron Corporation filed Critical Diatron Corporation
Priority to JP5516744A priority Critical patent/JPH07505467A/en
Priority to CA002132707A priority patent/CA2132707C/en
Priority to EP93908431A priority patent/EP0632887B1/en
Priority to DE69331629T priority patent/DE69331629T2/en
Priority to AT93908431T priority patent/ATE213832T1/en
Publication of WO1993019358A1 publication Critical patent/WO1993019358A1/en

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Classifications

    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N21/00Investigating or analysing materials by the use of optical means, i.e. using sub-millimetre waves, infrared, visible or ultraviolet light
    • G01N21/62Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light
    • G01N21/63Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light optically excited
    • G01N21/64Fluorescence; Phosphorescence
    • G01N21/6408Fluorescence; Phosphorescence with measurement of decay time, time resolved fluorescence
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N21/00Investigating or analysing materials by the use of optical means, i.e. using sub-millimetre waves, infrared, visible or ultraviolet light
    • G01N21/62Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light
    • G01N21/63Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light optically excited
    • G01N21/64Fluorescence; Phosphorescence
    • G01N21/645Specially adapted constructive features of fluorimeters
    • G01N2021/6463Optics
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N21/00Investigating or analysing materials by the use of optical means, i.e. using sub-millimetre waves, infrared, visible or ultraviolet light
    • G01N21/62Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light
    • G01N21/63Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light optically excited
    • G01N21/64Fluorescence; Phosphorescence
    • G01N21/645Specially adapted constructive features of fluorimeters
    • G01N21/6456Spatial resolved fluorescence measurements; Imaging

Definitions

  • This invention relates to detection of fluorescence from a solution or a surface. More particularly, this invention is adapted for measurement of transient state i ⁇ tmunoassays.
  • Fluorescence is the process of monitoring fluorescent radiation from an object for analysis, characterization or imaging.
  • an excitation pulse of radiation is directed onto or into a sample, followed by fluorescence of the sample, and the detection of the fluorescent radia ⁇ tion.
  • the detected fluorescence is used for sample analy ⁇ sis, characterization or imaging.
  • analysis of a sample is typically done by marking a desired species with a fluorescable tag, excit ⁇ ing the sample and monitoring for fluorescence from the tag.
  • fluorometry is capable of being the most sensitive of all analytic tools. It is possible to detect single photon events, and possible to re-excite a fluorophore and confirm the analysis.
  • the prob ⁇ lem which has plagued fluorescence has been in discrimi ⁇ nating the fluorescent signal of interest from the back ⁇ ground radiation in the system. Often times, the signal from "background" radiation may be 10,000 times larger than the intensity of the fluorescent signal of interest. Detection of the unwanted background radiation reduces the image quality and accuracy of the detection.
  • the problem caused by background radiation is particu- larly acute in biological systems.
  • a naturally occurring fluorescable material such as biliverdin
  • Other sources of undesirable background radiation include ambient radia ⁇ tion., radiation from fast fluorescing materials (generally considered to be those with decay half lives on the order of 1 to 1.5 nanoseconds) and various scattering mecha ⁇ nisms, such as Raman scattering bands.
  • a first technique involves discriminating against background radiation on the basis of wavelength.
  • a filter is used to reject detected radiation at all but a narrowly defined wavelength band. This technique has been less than successful principally because the background radia ⁇ tion may also be at the same wavelength as the desired fluorescence signal, and accordingly, still be passed through the filter and detected.
  • a second technique attempting to discriminate the desired fluorescent signal from the background is the so called time gating approach.
  • the fluorescent signal is observed in a short time window after the excitation.
  • the time window may be varied both in its length and in its starting time.
  • the detected radiation may be observed at the maximal time for detection sensitivity.
  • this technique has used a fluorophore of very long decay time (such as 1,000 nanoseconds) to allow the background fluorescence to substantially decay before detection of the fluorescent signal of interest.
  • long decay time fluorophores are less desirable than shorter decay time fluorophores because they are rela ⁇ tively insensitive and require longer times for overall analysis.
  • transient state fluorescent analysis utilizes a single, relatively high power pulse which excites the fluorophore.
  • the transient state is typically monitored by a high speed photomultiplier tube by monitoring the analog signal representative of current as a function of time.
  • Single pulse systems require suf ⁇ ficiently high power to excite a large number of fluores ⁇ cent molecules to make detection reliable.
  • the other principal format for transient state fluorescent analysis utilizes repetitive excitation pulses.
  • pulses of relatively short, typically nanosecond duration, light with power in the microwatt range are repetitively sup ⁇ plied to the sample at rates varying from 1 to 10,000 Hz.
  • the excitation source is a lamp, such as a Xenon-lamp.
  • the decay curve is measured digi ⁇ tally by determining the time to receipt of a photon.
  • One commercially available system uses repetitive pulses (such as at 5,000 Hz) and strobes the photomultiplier tube at increasingly longer times after the flash in order to obtain a time dependent intensity signal. Detection in such systems has proved to be very time consuming and insensitive. A single analysis can take on the order of one hour, even at relatively high fluorescable dye concen- trations (e.g. 10 "6 M) .
  • An improved fluorescence detection system utilizes a relatively high powered, relatively high repetition rate light source with high speed detection electronics to increase system sensitivity and accuracy.
  • the light source is a laser diode.
  • High speed detection elec- tronics permit single event photon counting.
  • a light source preferably a laser diode
  • Transient state detection is accomplished by repetitively exciting the fluorophore, and monitoring the number of events received by the detector within a defined time window.
  • Laser diodes are beneficially used as they have relatively high power (such as 5 to 100 milliwatts) , long lifetimes and may be pulsed at relatively high repetition rates (such as 10 MHz) . The combination of relatively high power excitation pulses plus relatively high repetition rates results in substantially quicker and more accurate fluorescent measurements.
  • a high powered light source preferably a laser diode
  • a high powered light source is used to obtain the decay profile of a fluorophore by measuring the time to receipt of a photon, and compiling a histogram from that data.
  • a hardware counter determines the total number of detection events within a monitor time. The shape of the fluorescence decay curve is determined by generating a histogram of time of receipt of photons.
  • a ramp voltage is sampled at time of event detection, and the voltage stored to compile a histogram. Once the preceding event is detected and the data stored, monitoring is resumed for detection of the next event.
  • the correct intensity may be determined by multiplication of the ratio of total number of events detected divided by the total number of events comprising the histogram.
  • the dark current is determined and subtracted from the total count and histogram count before the ratio is determined.
  • This technique permits direct generation of a histogram for which the data analysis techniques of Dandliker et al. , U.S. Patent No. 4,877,965 are directly applicable.
  • improved sensi ⁇ tivity is achieved by ignoring the data received immedi ⁇ ately after the excitation pulse.
  • the data acquisition window is set to start at a time after the initial transient events are concluded.
  • the data is acquired but not used during data analysis.
  • Fig. 1 shows an overview of the time gating transient state fluorescence decay measurement system.
  • Fig. 2 shows a block diagram of the time gating system.
  • Fig. 3 shows a representative timing diagram for aspects of the time gating system.
  • Fig. 4. shows a block diagram detail for the detector printed circuit board for the time gating system.
  • Fig. 5 shows a block diagram detail for the laser printed circuit board in the time gating system.
  • Fig. 6 shows a flow chart for the detection system in the time gating system.
  • Fig. 7 shows an overview of the fluorometer system for the detection of time of receipt of events.
  • Fig. 8 shows the block diagram detail for the data acquisition processor board for the time of detection system.
  • Fig. 9 shows a timing diagram for the time of detec- tion system.
  • Fig. 10 shows a detailed block diagram for the laser PCB of the time of detection system.
  • Fig. 11 shows a detailed block diagram of the detector printed circuit board for the time of detection system.
  • Fig. 12 is a flow chart for operation of the detec ⁇ tion system for the time of detection system.
  • Fig. 13 is a graph showing sensitivity and linearity utilizing the time of detection system, showing the log of the intensity of counts as a function of the log of the digoxin probe concentration.
  • Fig. 14 is a graph showing the digoxin serum assay utilizing the time of detection system, showing the raw data for the scatter and fluorescence curves, with inten- sity (counts/seconds) in thousands versus the time bin number.
  • Fig. 15 shows a graph of the timing system counter (counts/10 seconds) in thousands versus the high speed counter (counter/10 seconds) in millions for the time of detection system.
  • Fig. 16 shows a graph of the raw counts and normal ⁇ ized counts for time of detection system, with intensity in millions versus the probe concentration (moles per liters x 10 10 .
  • Fig. 17 shows a graph of transient-state polarization versus Digoxin concentration.
  • the intensity of fluorescence as a function of time may be quickly and accurately determined.
  • the system may measure either total intensity as a function of time, or may be config ⁇ ured to measure the intensity of the various polarization components of the signal as a function of time.
  • both steady state and transient state analysis is possi- ble.
  • transient state fluorescence is monitored in preference to steady state fluorescence.
  • Transient state fluorescence measure ⁇ ments tend to reduce the contribution from scatter bands and from fast fluorescers.
  • the systems of this invention com ⁇ prise a source of excitation radiation to be directed onto or into a sample, and a detection system for measuring fluorescence from the sample.
  • Conventional optics, such as filters and polarizers may be used in conjunction with the system of this invention as is well known to those skilled in the art.
  • the source of excitation radiation is characterized by being relatively high power and capable of operating at relatively high repetition rates.
  • a laser diode meets both of these requirements.
  • conventional laser diodes are available with power up to the 100 milliwatt range, which is roughly 1,000 times more powerful than conventional flash lamp fluorometers. It is expected that the power level of such devices will continue to increase. Further, conventional laser diodes may easily operate at 10 MHz range or higher, providing an over 1,000 times increase in the repetition rate as compared to flash lamp system and laser systems.
  • laser diodes are available in any number of discrete output wavelengths which are compatible with commercially available fluores- cent dyes.
  • laser diodes having wavelengths of 670 nm, 685 nm, 720 nm, 750 nm and 780 nm are avail ⁇ able.
  • Fluorescable dyes in these ranges may be manufac ⁇ tured in accordance with the teachings provided in the application to Arrhenius and Dandliker and Hsu, incorpo- rated by reference above, and in Fluorescence Immunoassays Using Fluorescent Dyes Free of Aggregation and Serum Bind ⁇ ing, filed on the same day as the instant application, and incorporated herein by reference.
  • caged dicarboxy silicon phthocyanines When a digoxin probe is used, it is referred to as caged dicarboxy silicon phthocyanine-digoxigenin.
  • a digoxin probe When a digoxin probe is used, it is referred to as caged dicarboxy silicon phthocyanine-digoxigenin.
  • tunable laser diodes may be used in conjunction with this invention.
  • quantum well diodes provide the capability of tuning the output wavelength.
  • the detection system generally permits the detection of single photon events. High bandwidth devices are com ⁇ flashally available and are utilized to monitor detected events.
  • Fig. 1 shows an overview of one embodiment of this invention.
  • the decay profile of the fluorophore is obtained by varying a time window, either or both as to its starting time or as to its duration.
  • the main components comprise an excitation source, a sam ⁇ ple holder, related optics, and a detector.
  • Optional processing and display capabilities are provided, for example, by a computer.
  • the laser driver PCB 10 contains, preferably, the laser diode and certain optics.
  • the laser driver PCB 10 is preferably rotatable such that the polarization orientation of the diode laser may be varied.
  • the laser diode (not shown) on the laser driver PCB 10 is directed to the reaction cell 16 to cause excitation of the material contained within the reaction cell 16.
  • the fluorescent radiation is detected by the detector PCB 12.
  • the detector is oriented at right angles from the input radiation.
  • the main PCB 14 connects to the laser driver PCB 10 and detector PCB 12, plus communication with the computer 18.
  • optics may be placed within the path of the light, such as filters 20, lens 22, and/or aperture 24.
  • Various combina- tions of polarizers may be utilized, as is well known to those skilled in the art, including rotatable polarizers 26 which is controlled both from the main PCB 14.
  • the reaction cell 16 may be provided with a stirrer, most preferably a magnetic type stirrer.
  • the computer 18 provides one way in which the user may interface with the system for control, processing, and display functions.
  • the computer 18 may be either of a stand-alone type, or its necessary functions may be imple ⁇ mented with a collection of discreet components as is known to those skilled in the art.
  • the computer 18 is Fig.
  • the computer 18 may control numerous functions, it provides control for functions such as: laser on-time, laser power, laser on-off control, PMT high voltage set point, PMT current detection threshold set point, PMT on-off, delay to start of detection window, delay to end of detection window, number of cycles per experiment, polarizer parallel-perpendicular, stirrer on-off, and laser diode operating temperature.
  • Fig. 2 shows a detailed block diagram of the main PCB 14.
  • a microprocessor 30 controls operation of the board.
  • a microprocessor 30 is an 80C32 processor and the memory 32 is 32K bytes of ROM and 32 K bytes of RAM.
  • an interface 34 such as an RS232 port, permits connection to a computer for display 36.
  • the microprocessor 30 pro ⁇ vides control signals for the high voltage power supply control, the threshold comparator voltage control, and the polarizer motor.
  • the polarizer motor (not shown) serves to rotate the polarizer to permit detection of various polarization orientations.
  • the excitation source is provided by the laser and optics block 40. Excitation light irradiates the sample 42, and fluorescent radiation is passed through the optics and polarizer 44 to the detector 46.
  • the microprocessor 30 sets the timer/ master counter 50 to set the on time for the laser 40, and the laser off counter 52 to determine the time at which the laser 40 is turned off.
  • the microprocessor 30 further sets the window open counter 54 to correspond to the open- ing of the data acquisition window and sets window closed counter 56 to correspond to the closing of the data acqui ⁇ sition window.
  • a gate 58 receives the output of the detector 46 and passes it to the counter 60 during the data acquisition window.
  • Control for the gate 58 comes from the window open counter 54, which permits passage of pulses from the detector 46 to the counter 60, and the window closed counter 56 which closes the gate 58, pre- eluding data from passing from the detector 46 to the counter 60.
  • the value of counts in the counter 60 is transferred under control of the micropro ⁇ cessor 30 to memory 32 for later processing, analysis, and display.
  • Fig. 3 shows the general timing aspects of the cir ⁇ cuit of Fig. 2.
  • a system clock 62 provide overall system synchronization and control.
  • An example for the system clock frequency might be 10 MHz.
  • the cycle time is 100 ns, giving a maximum 50 ns on period.
  • the laser pulse duration is controlled by the timer/master counter 50 and laser off counter 52.
  • the leading edge of the system clock 62 triggers the genera ⁇ tion of the laser pulse 64.
  • the trailing edge of the laser pulse is determined by the time set in the laser off counter 52.
  • the waveform 66 of Fig. 3 shows the laser-off counter state, transitioning low when the laser pulse 64 is to terminate.
  • the window open counter pulse 68 runs for a time until the beginning of the data acquisition window 72.
  • the window closed counter pulse 70 runs longer than the window open counter pulse 68, the trailing edge of the window closed counter pulse 70 defining the trail ⁇ ing edge of the data acquisition window pulse 72.
  • the data acquisition window pulse 72 defines the time period in which the data is supplied from the detector 46
  • the composite fluorescence signal 74 has an initial steady state portion 76 followed by an intensity decay portion 78. In actuality, for any given single laser pulse, it is more probable than not that no photon will be detected for any data acquisition window. Accordingly, the fluorescence signal 74 would be a compilation of events after numerous laser pulses run with various data acquisition window times.
  • Fig. 4 shows the detail of the detector PCB 12.
  • detection electronics capable of detecting single photon events are used.
  • a photomultiplier tube (“PMT") 80 is oriented to detect the fluorescence from a sample (not shown) .
  • the PMT 80 has a low dark current and a high band width, such as 100 MHz.
  • a high voltage power supply 82 supplies power to the PMT 80.
  • a high voltage power supply control signal 84 from the main PCB 14 (shown on Fig. 2) determines the value of high voltage supply from the power supply 82 to the PMT 80.
  • the output of the PMT 80 is amplified as is necessary.
  • a comparator 88 allows for selection of the desired pulse amplitude and compensates for offsets in the amplifier 86.
  • the compara ⁇ tor 88 is preferably controlled by a threshold comparator voltage control (from Fig. 2) .
  • the output of the compara ⁇ tor 88 goes to the counter 60 (Fig. 2) via gate 58.
  • the cable connection from the main PCB 14 to the detector PCB 12 is a 65 ohm shielded ribbon cable whose length is kept less than 12 inches.
  • Fig. 5 shows the detail of the laser PCB 10.
  • Laser diode 90 is preferably housed in a beam collimator 92 and mounted directly on laser PCB 10.
  • a socket assembly may be used to ease in changing laser diodes 90.
  • the collimator assembly 92 and laser diode 90 are further housed within a sealed compart ⁇ ment 94 with a desiccant (not shown) .
  • Temperature control circuit 96 monitors the temperature of the laser diode 90 via a thermistor 98.
  • a heater 100 is controlled by the temperature control 96 to heat the laser diode 90.
  • the temperature set point control determines the temperature at which the temperature control 96 regulates.
  • a laser diode driver 102 provides driving power to the laser diode 90. Control inputs to the laser diode driver 102 include the laser on-off control and laser power level set, both of which come from the main PCB 14.
  • the laser diode 90 is operated at 10 MHz pulse repetition rate and at peak power approximately 6 to 7 times the average rated power output. Exceeding the rated power on a peak basis is possible because the laser pulses are so short that the normal failure mecha- nism, thermal mirror failure, does not occur since the average power is less than the typical continuous operat ⁇ ing power.
  • Fig. 6 shows a flow chart for the overall operation.
  • the microprocessor 30 sets the laser on time 104 and laser off time 106.
  • the delay time to the beginning of the data acquisition window is set by the microprocessor 30 and is labeled as start delay 108.
  • pulses exceeding the threshold level as set by the microprocessor 30 are counted at step 110. These events are summed as count 112.
  • the decisional block 114 directs the re-initiation of the cycle, causing another laser pulse and counting to begin.
  • the results are provided to the computer or other data processing device.
  • a histogram of intensity as a function of time may be compiled.
  • the data collection and analysis techniques of Dandliker et al. United States Patent No. 4,877,965 are preferably used to further improve the quality of the data.
  • the timing resolution of the system may be set as precisely as desired. In the preferred embodiment, a timing resolution of 400 picoseconds was selected to permit accurate formation of fluorescent decay times as short as 2 nanoseconds. The data acquisition window is then taken as multiples of the timing resolution value.
  • Fig. 7 shows a systemwide view of a fluorometer in accordance with this invention designed to determine the time of detection of a photon. After numerous repetitions of the detection cycle, a histogram of the number of events as a function of time is developed. In the pre ⁇ ferred embodiment, data is collected for time bins, for •example, 1,024 time bins or intervals over 75 nanoseconds results in a bin width of 75 picoseconds.
  • a laser PCB and input optics board 120 generates and directs a laser beam towards a reaction cell 124.
  • Fluorescent light from the reaction cell 124 is detected by the detector PCB 126, whose output is amplified by the amplifier PCB 130, whose signal in turn is supplied to the comparator PCB 132, with the ultimate result being supplied to the data acquisition PCB 128.
  • the result from the data acquisition PCB 128 may be provided to a computer 134 or other functionally simi ⁇ lar data processing device.
  • an interface PCB 136 provides connection between the data acquisition PCB 128 and the laser PCB 120.
  • a thermal control PCB 138 monitors and controls the temperature of the laser diode (not shown) .
  • optional filters 140, polarizer 142 , lens 144, and aperture 146 may be used as known to those skilled in the art and described previously in connection with the embodiment described above.
  • the laser PCB 120 provides a sequence of laser pulses to the reaction cell 124.
  • the detector PCB 126 detects receipt of photons, if any, and after amplified by amplifier PCB 130, for the signal which exceeds the level set for the comparator PCB 132, an event is considered detected by the data acquisition PCB 128.
  • the detection of an event is then used in two ways. First, a running count of the total number of events is made for the time period of interest. In a preferred embodiment, the time period of interest runs continuously during the detection period. Secondly, the detection of an event is used to determine the time at which the event occurred.
  • the microprocessor 140 and memory 42 operate on the data acquisition PCB 128 to control the system.
  • an interface 144 such as an RS 232 port, permits connection with a computer 146 or other data processing or display device.
  • the microprocessor 140 provides numerous control signals, such as: control to the polarizer control 128, the PMT high voltage control, and the ICONT signal, typi ⁇ cally via digital to analog convertors 150.
  • An overall clock signal 152 is preferably on the order of 10 MHz. This provides a 100 nanosecond cycle time.
  • the timing circuit 154 generates a laser drive pulse 156 which causes generation of the laser pulse hav ⁇ ing a shape 160.
  • the timing circuit 154 further causes activation of a delay circuit 156 which in turn, after a predetermined delay, activates ramp generator 158.
  • the ramp voltage 162 begins with a period of delay (see Fig. 9) and then begins a ramp portion. In a preferred embodiment, the delay period is 25 nanoseconds.
  • the value of the ramp voltage 162 is latched, such as by flip-flop 166.
  • the latched value of voltage from the ramp generator 158 is converted in an analog to digital converter 168 and provided to microprocessor 140 for storage in memory 142. Additionally, the detect event signal 164 is provided to counter 170 which maintains a running count of all detected events.
  • the counter 170 counts all events detected, no matter when in the cycle they are detected. Specifically, the counter 170 counts detected events whether during the dark current period, during the laser pulse time, or during the transient state fluores ⁇ cent decay period. Alternatively, the counter 170 may be activated only during desired times, for example, being inactivated during the dark current time.
  • a detected event 164 is received by the data acquisition PCB 128 (Fig. 8) . While this process is ongoing, the time detection system ignores new photons or events until the previously received photon time has been completed. Depending upon the particular hardware chosen, the time during which new photons are ignored can be on the order of 30 microseconds. If the clock frequency is 10 MHz, approximately 300 laser pulses are ignored. Gen ⁇ erally, this is insignificant in all but the highest con ⁇ centration of fluorophores. At nominal concentrations, typical input rates of photon events from the PMT is approximately 10,000 per second. Accordingly, a photon is detected roughly every 1,000 pulses.
  • pulse rates may increase by orders of magnitude.
  • laser diode peak power may be lowered or apertures may be placed in the detection path.
  • the counter 170 monitors all detected events, independent of the timing of the detected event.
  • the shape of the histogram may be determined by measuring the time of the detected event for a large number of samples.
  • the counter 170 provides for the calculation of a scale factor so as to provide a true measure of the intensity of the fluorophore decay as a function of time.
  • the dark current signal level (the level of cur ⁇ rent or detected events existing even with no laser pulse or fluorescent decay) is detected.
  • the value of the dark current is subtracted from the total number of counts in each bin. In this way, a true measure of the number of detected events occurring during that time bin is set.
  • the total number of counts in the time bins are summed, giving a measure of the total number of events detected.
  • the ratio of events counted by counter 170 and the number of events found by integrating all of the bin counts is multiplied times the value in each bin. In this way, compensation is made for events which occurred during the analysis, as indi ⁇ cated by a detected event stored by counter 170, but which did not form part of the histogram as detected by the sampling of values from the ramp voltage 162 (presumably because an event was being processed) .
  • the laser PCB 120 takes the laser drive pulse 158 from the data acquisition processor board
  • the duration of the pulse is on the order of a few nanoseconds, and is of relatively high power.
  • An incoming rising edge in the laser drive pulse 158 causes generation of a laser flash.
  • Input logic 170, 174, and 176 generate a very sharp rising edge, which is supplied to the high-powered digital driver 178.
  • the digital driver 178 provides power to the laser diode 180.
  • the current used by the laser diode 180 is set by the signal ICONT from the data acquisition PCB (Fig. 8) .
  • the duration of the laser pulse may be varied by changing the delay 172. Further, the amplitude of the laser pulse is varied by setting the current value ICONT.
  • a reference diode 182 monitors the long term stability of the laser output.
  • the reference diode 182 is located downstream of the optics and filter through which the laser beam passes. In this way, the total input power directed to the sample may be monitored. Various factors which affect total input power would include laser perfor ⁇ mance or degradation, cleanliness of the optical compo ⁇ nents or degradation of the laser filter.
  • a photocurrent monitor 184 monitors the photocurrent of the laser diode 180. Since the pulse length and repetition rate are known, the average power being generated by the laser diode 180 may be calculated. This power reading, labeled VMON, is fed back to the data acquisition PCB (Fig. 8) .
  • an optional heater 186 and thermistor and temperature control 188 provide temperature control to the laser diode 180.
  • the temperature set point is provid ⁇ ed from the data acquisition PCB to the heater 186 and control 188.
  • varying the temperature changes the wavelength of the laser diode 180.
  • the detector PCB 126 is described in detail in Fig. 11.
  • the photomultiplier tube 190 receives fluores ⁇ cent radiation from the sample.
  • a high voltage generator 192 under control the PMT high voltage control signal 194 as amplified 196 provides high voltage to the PMT 190.
  • the output of the PMT 190 is passed through amplifier 192 and sent through comparator 194.
  • the compara ⁇ tor passes the signal as output to the data acquisition PCB.
  • the amplifier 192 is connected to the comparator 194 by dual coaxial cable providing a differen ⁇ tial signal.
  • the comparator 194 is similarly connected via coaxial cables to the data acquisition PCB.
  • Fig. 12 shows a flow chart for the preferred method of operation. During the initialization phase 200, the following items are set: the PMT voltage, laser intensi ⁇ ty, data acquisition time, liquid crystal polarizer ("LCP”) cycles, and LCP to parallel.
  • LCP liquid crystal polarizer
  • the ramp voltage is frozen 212 and the height measured and converted to digital 214.
  • the polarizer may be changed to the other orientation instead 222.
  • the fluorometry system described herein when used in conjunction with the fluorescable dyes described in copending applications to Arrhenius and Dandliker and Hsu result in an improvement in signal detection of over 100 times over conventional techniques.
  • the following table lists the detectable concentration level of dye at the point where the intensity of the desired signal equals the intensity of the background.
  • the buffer used contains 1% bovine serum albumin. The data are as follows:
  • Fig. 13 shows a log-log plot of the intensity as a function of Digoxin probe concentration. The results show the system to be linear over four orders of magnitude. Further, concentrations as low as approxi ⁇ mately IO "13 moles per liter may be detected. An accurate system should have such a linear response, since as the concentration of fluorescable material decreases, there should be a correspondingly linear decrease in the number of counts detected.
  • Fig. 14 Actual data from a sample is shown in Fig. 14.
  • the intensity (number of counts per 10 seconds) is shown on the y-axis measured in thousands.
  • the x-axis shows the time bin number, with each bin corresponding to a 75 pico ⁇ second interval.
  • the scatter curve peaks slightly to the left of the peak of the fluorescence curve.
  • the dark current counts are shown generally in the time from bin number 200 to bin number approximately 300.
  • the decay of the fluorescence curve as a function of time provides a histogram which may be used in conjunction with data analysis techniques such as those disclosed in Dandliker et al. U.S. Patent No. 4,877,965.
  • the time of detection system forms a histogram which accurately depicts the shape of the intensity curve, and then scales that shape to provide an absolute measure of intensity as a function of time.
  • the method used is to monitor the total number of counts with a high speed hardware counter and to determine the total number of counts comprising the shape histogram by integrating those counts.
  • the histogram shape curve is then multiplied by the ratio of the hardware counts to the total integrated counts.
  • Fig. 15 shows the integrated timing system counts as a function of high speed counter counts. A maximum of 33,000 counts per second may be detected by the timing system counter. This however is a function of the speci ⁇ fic hardware chosen. If a dedicated processor or faster processor were chosen, as are design choices available to those skilled in the art, the time required to store a time of receipt of an event is decreased, and accordingly, the number of counts per second may be increased.
  • Fig. 16 shows the intensity (in millions) as a func ⁇ tion of probe concentration (in moles per liter x 10 10 ) for two curves.
  • the upper curve shows the normalized counts and the lower curve shows the raw counts.
  • the raw counts may be in ⁇ verted into normalized counts, thereby providing liner . y of intensity as a function of probe co.-. entraci n.
  • the photon flux is relatively low.
  • Fig. 17 shows a graph of transient-state polarization versus digoxin concentration.
  • a 20 microliter sample containing known levels of digoxin were incubated with 25 microliters of rabbit anti- digoxin antibody for 5 minutes in 100 microliter of buf- fer.
  • the 20 microliters of fluorescently labelled digoxin probe (at a concentration 5 x 10 "11 M was then added and incubated for an additional 5 minutes.
  • the solu ⁇ tions were diluted with 1 milliliter of buffer. The fluorescence signal was then read using the time of detec- tion hardware apparatus.

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Abstract

An improved fluorescence detection system is provided which utilizes a relatively high powered, relatively high repetition rate light source (10) with high speed detection electronics to increase system sensitivity and accuracy. In the preferred embodiments, a laser diode (90) is the light source (10). In one embodiment, the position of a time window is varied to compile a decay profile of a fluorophore. In another embodiment, the time of detection of a photon is used to compile the decay profile. In one aspect of this invention, a histogram of the fluorescence decay is generated by determining a preliminary histogram of the shape and multiplying it by the ratio of the total number of events divided by the number of events comprising the preliminary histogram. In another aspect of this invention, the time of detection after excitation of the photon is started from a random time, such as after a preceding event is detected and the data stored.

Description

DESCRIPTION
FLUOROMETER DETECTION SYSTEM
Field of the Invention
This invention relates to detection of fluorescence from a solution or a surface. More particularly, this invention is adapted for measurement of transient state iπtmunoassays.
Background of the Invention
Fluorescence is the process of monitoring fluorescent radiation from an object for analysis, characterization or imaging. Typically, an excitation pulse of radiation is directed onto or into a sample, followed by fluorescence of the sample, and the detection of the fluorescent radia¬ tion. The detected fluorescence is used for sample analy¬ sis, characterization or imaging. In the case of an immunoassay, analysis of a sample is typically done by marking a desired species with a fluorescable tag, excit¬ ing the sample and monitoring for fluorescence from the tag.
Theoretically, fluorometry is capable of being the most sensitive of all analytic tools. It is possible to detect single photon events, and possible to re-excite a fluorophore and confirm the analysis. However, the prob¬ lem which has plagued fluorescence has been in discrimi¬ nating the fluorescent signal of interest from the back¬ ground radiation in the system. Often times, the signal from "background" radiation may be 10,000 times larger than the intensity of the fluorescent signal of interest. Detection of the unwanted background radiation reduces the image quality and accuracy of the detection.
The problem caused by background radiation is particu- larly acute in biological systems. For example, in the analysis of blood plasma, the presence of a naturally occurring fluorescable material, such as biliverdin, causes substantial background radiation. Other sources of undesirable background radiation include ambient radia¬ tion., radiation from fast fluorescing materials (generally considered to be those with decay half lives on the order of 1 to 1.5 nanoseconds) and various scattering mecha¬ nisms, such as Raman scattering bands.
Earlier attempts to overcome the problem of backg¬ round radiation have met with limited success. A first technique involves discriminating against background radiation on the basis of wavelength. Generally, a filter is used to reject detected radiation at all but a narrowly defined wavelength band. This technique has been less than successful principally because the background radia¬ tion may also be at the same wavelength as the desired fluorescence signal, and accordingly, still be passed through the filter and detected.
A second technique attempting to discriminate the desired fluorescent signal from the background is the so called time gating approach. Here, the fluorescent signal is observed in a short time window after the excitation. The time window may be varied both in its length and in its starting time. Through the use of the variable time window, the detected radiation may be observed at the maximal time for detection sensitivity. Historically, this technique has used a fluorophore of very long decay time (such as 1,000 nanoseconds) to allow the background fluorescence to substantially decay before detection of the fluorescent signal of interest. Generally however, long decay time fluorophores are less desirable than shorter decay time fluorophores because they are rela¬ tively insensitive and require longer times for overall analysis.
Historically, there have been two excitation pulse formats for transient state fluorescent analysis. One format utilizes a single, relatively high power pulse which excites the fluorophore. The transient state is typically monitored by a high speed photomultiplier tube by monitoring the analog signal representative of current as a function of time. Single pulse systems require suf¬ ficiently high power to excite a large number of fluores¬ cent molecules to make detection reliable. The other principal format for transient state fluorescent analysis utilizes repetitive excitation pulses. Ordinarily, pulses of relatively short, typically nanosecond duration, light with power in the microwatt range are repetitively sup¬ plied to the sample at rates varying from 1 to 10,000 Hz. Ordinarily, the excitation source is a lamp, such as a Xenon-lamp. Frequently, the decay curve is measured digi¬ tally by determining the time to receipt of a photon. One commercially available system uses repetitive pulses (such as at 5,000 Hz) and strobes the photomultiplier tube at increasingly longer times after the flash in order to obtain a time dependent intensity signal. Detection in such systems has proved to be very time consuming and insensitive. A single analysis can take on the order of one hour, even at relatively high fluorescable dye concen- trations (e.g. 10"6M) .
Recently, significant advances have been made in the area of fluorescable dyes. In one aspect, dyes being excitable by longer wavelength radiation, such as in the red and infrared wavelengths, are now available. Appli- cant incorporates by reference the applications by Arrhenius, U.S. Patent Application Serial No. 701,449, filed May 15, 1991, entitled, "Fluorescent Marker Compo¬ nents and Fluorescent Probes" (which is a continuation-in- part of U.S. Patent Application No. 523,601, filed May 15, 1990) , and Dandliker and Hsu, U.S. Patent Application Serial No. 701,465, filed May 15, 1991, entitled "Fluores¬ cent Dyes Free of Aggregation and Serum Binding" (which is a continuation-in-part of U.S. Patent Application Serial No. 524,212, filed May 15, 1990) . Significant improve- ments in sensitivity are achieved through use of these modern dyes over older dyes. Further significant advancements have been made in increasing sensitivity through data collection and analy¬ sis techniques. As disclosed in Dandliker et al. , U.S. Patent No. 4,877,965, entitled "Fluorometer, " time gating techniques are used in conjunction with data collection and analysis techniques to obtain an improved signal rela¬ tive to the background. Generally, Dandliker et al. , con¬ siders the detected intensity as a function of time to be composed of signals from various sources, including the desired signal source, and various undesired background sources. Optimization of the desired signal is achieved through data collection and analysis techniques.
Further significant advancements have been made in the ability to measure relevant materials in immunoassays. For example, in Dandliker et al, U.S. Patent Application Serial No. 490,770, filed March 6, 1990, entitled "Tran¬ sient State Luminescence Assays" (which is a continuation- in-part of U.S. Patent Application No. 365,420, filed June 13, 1989) incorporated herein by this reference, the bound and free form of materials in a homogeneous assay may be determined. Generally, the technique requires measurement of the time dependent decay of the intensity of parallel and perpendicular polarization components. By measuring the time dependent decay of various polarization states, it is possible to determine the bound and free forms of materials such as haptens, peptides, or small proteins in a homogeneous analysis format. Significantly, no separa¬ tion of the bound and free materials is required.
Despite the significant and promising improvements made in the field of fluorescable dyes, and in the data analysis aspects, the actual methods and apparatus for achieving and detecting fluorescence have heretofore remained relatively unchanged. Utilizing even the most sensitive and best equipment, analysis can take an hour or more, even at high concentrations of materials. When fluorometry is used for immunoassay in a clinical context, time for analysis and proper diagnosis can be absolutely critical. Patient survival can depend on accurate, timely analysis. Additionally, rapid testing would permit retests of patients without having them wait significant periods of time, resulting in more rapid and accurate diagnosis. As to sensitivity, it is extremely desirable to be able to detect minute amounts of fluorescable mater¬ ial. However, as the amount of fluorescable material in a sample decreases, the ratio of the size of the undesired background signal to the desired signal increases. Fur- ther, since the time for analysis depends on the amount of fluorescent radiation received from the detector, low con¬ centrations generally require substantially more time to analyze.
Heretofore, the time required for analysis has been prohibitively high. Known methods and apparatus have failed to provide rapid and accurate diagnosis and analy¬ sis of samples. This has been so despite the clear and known desirability of the use of fluorometry.
Summary of the Invention An improved fluorescence detection system utilizes a relatively high powered, relatively high repetition rate light source with high speed detection electronics to increase system sensitivity and accuracy. Preferably, the light source is a laser diode. High speed detection elec- tronics permit single event photon counting.
In one embodiment, a light source, preferably a laser diode, is used to obtain the decay profile of a fluoro¬ phore by varying a position of a time window. Transient state detection is accomplished by repetitively exciting the fluorophore, and monitoring the number of events received by the detector within a defined time window. Laser diodes are beneficially used as they have relatively high power (such as 5 to 100 milliwatts) , long lifetimes and may be pulsed at relatively high repetition rates (such as 10 MHz) . The combination of relatively high power excitation pulses plus relatively high repetition rates results in substantially quicker and more accurate fluorescent measurements.
In a preferred embodiment, a high powered light source, preferably a laser diode, is used to obtain the decay profile of a fluorophore by measuring the time to receipt of a photon, and compiling a histogram from that data. A hardware counter determines the total number of detection events within a monitor time. The shape of the fluorescence decay curve is determined by generating a histogram of time of receipt of photons. In the preferred embodiment, a ramp voltage is sampled at time of event detection, and the voltage stored to compile a histogram. Once the preceding event is detected and the data stored, monitoring is resumed for detection of the next event. After the shape of the decay curve is determined, the correct intensity may be determined by multiplication of the ratio of total number of events detected divided by the total number of events comprising the histogram. Preferably, the dark current is determined and subtracted from the total count and histogram count before the ratio is determined. This technique permits direct generation of a histogram for which the data analysis techniques of Dandliker et al. , U.S. Patent No. 4,877,965 are directly applicable. In another aspect of this invention, improved sensi¬ tivity is achieved by ignoring the data received immedi¬ ately after the excitation pulse. In one embodiment, the data acquisition window is set to start at a time after the initial transient events are concluded. In another embodiment, the data is acquired but not used during data analysis.
Accordingly, it is a principal object of this inven¬ tion to provide an improved fluorometer with greatly enhanced sensitivity. It is yet another object of this invention to provide a fluorometer capable of generating rapid and accurate determinations, often within a matter of seconds. It is yet a further object of this invention to provide a system capable of measuring extremely low concentrations of fluorescable material.
It is an object of this invention to provide a fluo- rometer useful for the clinical setting in that it is relatively compact, of relatively low cost and relatively rugged.
It is a further object of this invention to provide a fluorometer particularly adapted to exploit the new generation, longer wavelength fluorescable dyes.
Brief Description of the Drawings
Fig. 1 shows an overview of the time gating transient state fluorescence decay measurement system.
Fig. 2 shows a block diagram of the time gating system.
Fig. 3 shows a representative timing diagram for aspects of the time gating system.
Fig. 4. shows a block diagram detail for the detector printed circuit board for the time gating system. Fig. 5 shows a block diagram detail for the laser printed circuit board in the time gating system.
Fig. 6 shows a flow chart for the detection system in the time gating system.
Fig. 7 shows an overview of the fluorometer system for the detection of time of receipt of events.
Fig. 8 shows the block diagram detail for the data acquisition processor board for the time of detection system.
Fig. 9 shows a timing diagram for the time of detec- tion system.
Fig. 10 shows a detailed block diagram for the laser PCB of the time of detection system.
Fig. 11 shows a detailed block diagram of the detector printed circuit board for the time of detection system. Fig. 12 is a flow chart for operation of the detec¬ tion system for the time of detection system.
Fig. 13 is a graph showing sensitivity and linearity utilizing the time of detection system, showing the log of the intensity of counts as a function of the log of the digoxin probe concentration.
Fig. 14 is a graph showing the digoxin serum assay utilizing the time of detection system, showing the raw data for the scatter and fluorescence curves, with inten- sity (counts/seconds) in thousands versus the time bin number.
Fig. 15 shows a graph of the timing system counter (counts/10 seconds) in thousands versus the high speed counter (counter/10 seconds) in millions for the time of detection system.
Fig. 16 shows a graph of the raw counts and normal¬ ized counts for time of detection system, with intensity in millions versus the probe concentration (moles per liters x 1010. Fig. 17 shows a graph of transient-state polarization versus Digoxin concentration.
Detailed Description
In accordance with this invention, the intensity of fluorescence as a function of time may be quickly and accurately determined. The system may measure either total intensity as a function of time, or may be config¬ ured to measure the intensity of the various polarization components of the signal as a function of time. Further, both steady state and transient state analysis is possi- ble. However, in the preferred embodiment, transient state fluorescence is monitored in preference to steady state fluorescence. Transient state fluorescence measure¬ ments tend to reduce the contribution from scatter bands and from fast fluorescers. Broadly speaking, the systems of this invention com¬ prise a source of excitation radiation to be directed onto or into a sample, and a detection system for measuring fluorescence from the sample. Conventional optics, such as filters and polarizers may be used in conjunction with the system of this invention as is well known to those skilled in the art.
The source of excitation radiation is characterized by being relatively high power and capable of operating at relatively high repetition rates. A laser diode meets both of these requirements. Generally, conventional laser diodes are available with power up to the 100 milliwatt range, which is roughly 1,000 times more powerful than conventional flash lamp fluorometers. It is expected that the power level of such devices will continue to increase. Further, conventional laser diodes may easily operate at 10 MHz range or higher, providing an over 1,000 times increase in the repetition rate as compared to flash lamp system and laser systems. Currently, laser diodes are available in any number of discrete output wavelengths which are compatible with commercially available fluores- cent dyes. For example, laser diodes having wavelengths of 670 nm, 685 nm, 720 nm, 750 nm and 780 nm are avail¬ able. Fluorescable dyes in these ranges may be manufac¬ tured in accordance with the teachings provided in the application to Arrhenius and Dandliker and Hsu, incorpo- rated by reference above, and in Fluorescence Immunoassays Using Fluorescent Dyes Free of Aggregation and Serum Bind¬ ing, filed on the same day as the instant application, and incorporated herein by reference. These dyes are gener¬ ally referred to as caged dicarboxy silicon phthocyanines, and when a digoxin probe is used, it is referred to as caged dicarboxy silicon phthocyanine-digoxigenin. Fur¬ ther, it is possible to overdrive the laser diodes in order to increase their power output, provided that they are not overheated to cause damage to the diode. Further, tunable laser diodes may be used in conjunction with this invention. For example, quantum well diodes provide the capability of tuning the output wavelength. The detection system generally permits the detection of single photon events. High bandwidth devices are com¬ mercially available and are utilized to monitor detected events. The particular embodiments described below have been found to be particularly advantageous in connection with the detection methods described herein. Signifi¬ cantly, ultra high-speed events may be measured with detection electronics of significantly lower operating speed. An important aspect of this invention is to perform fluorescent determinations on samples which are relatively unaffected by background events. Significant improvement in detection of desired fluorescence signal may be achieved by excluding the extremely transitory events from consideration. As detailed in the Experimental Results section, below, an improvement of approximately 100 times over conventional methods is achieved. This exclusion may be achieved in any number of ways. The data may be excluded by the time gating technique, for example, by setting the time gate to begin after the extremely transi¬ tory events are substantially concluded. Alternatively, the data may be collected but not considered during the analysis of the data. Further, the polarization of the radiation may be monitored, thereby permitting data analy- sis. Significant improvements in the sensitivity of the system may be achieved through this technique.
Overall r significant improvements in speed of analy¬ sis and sensitivity are achieved by the systems of this invention. By increasing the repetition rate and the power of the excitation pulses each by a factor of approx¬ imately 1,000, substantial improvements are made in detec¬ tion sensitivity and drastically reduce the time for analysis. Detection may be done in a matter of seconds which previously would take hours. Further, use of fast detection electronics permits counting of single photon events, yet further increasing the sensitivity and accura¬ cy of the system. Fig. 1 shows an overview of one embodiment of this invention. The decay profile of the fluorophore is obtained by varying a time window, either or both as to its starting time or as to its duration. Structurally, the main components comprise an excitation source, a sam¬ ple holder, related optics, and a detector. Optional processing and display capabilities are provided, for example, by a computer.
In the preferred embodiment, there are three main printed circuit boards, the laser driver PCB 10, the detector PCB 12, and the main PCB 14. The laser driver PCB 10 contains, preferably, the laser diode and certain optics. The laser driver PCB 10 is preferably rotatable such that the polarization orientation of the diode laser may be varied. The laser diode (not shown) on the laser driver PCB 10 is directed to the reaction cell 16 to cause excitation of the material contained within the reaction cell 16. The fluorescent radiation is detected by the detector PCB 12. Preferably, the detector is oriented at right angles from the input radiation. The main PCB 14 connects to the laser driver PCB 10 and detector PCB 12, plus communication with the computer 18. Optionally, optics may be placed within the path of the light, such as filters 20, lens 22, and/or aperture 24. Various combina- tions of polarizers may be utilized, as is well known to those skilled in the art, including rotatable polarizers 26 which is controlled both from the main PCB 14. Option¬ ally, the reaction cell 16 may be provided with a stirrer, most preferably a magnetic type stirrer. The computer 18 provides one way in which the user may interface with the system for control, processing, and display functions. The computer 18 may be either of a stand-alone type, or its necessary functions may be imple¬ mented with a collection of discreet components as is known to those skilled in the art. The computer 18 is Fig. 1 is shown with a characteristic display of a tran¬ sient state decay of a fluorophore as a function of time. While the computer 18 may control numerous functions, it provides control for functions such as: laser on-time, laser power, laser on-off control, PMT high voltage set point, PMT current detection threshold set point, PMT on-off, delay to start of detection window, delay to end of detection window, number of cycles per experiment, polarizer parallel-perpendicular, stirrer on-off, and laser diode operating temperature.
Fig. 2 shows a detailed block diagram of the main PCB 14. A microprocessor 30 controls operation of the board. In a preferred embodiment, a microprocessor 30 is an 80C32 processor and the memory 32 is 32K bytes of ROM and 32 K bytes of RAM. Optionally, an interface 34, such as an RS232 port, permits connection to a computer for display 36. While not shown directly, the microprocessor 30 pro¬ vides control signals for the high voltage power supply control, the threshold comparator voltage control, and the polarizer motor. The polarizer motor (not shown) serves to rotate the polarizer to permit detection of various polarization orientations.
The excitation source is provided by the laser and optics block 40. Excitation light irradiates the sample 42, and fluorescent radiation is passed through the optics and polarizer 44 to the detector 46. In operation, the microprocessor 30 sets the timer/ master counter 50 to set the on time for the laser 40, and the laser off counter 52 to determine the time at which the laser 40 is turned off. The microprocessor 30 further sets the window open counter 54 to correspond to the open- ing of the data acquisition window and sets window closed counter 56 to correspond to the closing of the data acqui¬ sition window. A gate 58 receives the output of the detector 46 and passes it to the counter 60 during the data acquisition window. Control for the gate 58 comes from the window open counter 54, which permits passage of pulses from the detector 46 to the counter 60, and the window closed counter 56 which closes the gate 58, pre- eluding data from passing from the detector 46 to the counter 60. Periodically, the value of counts in the counter 60 is transferred under control of the micropro¬ cessor 30 to memory 32 for later processing, analysis, and display.
Fig. 3 shows the general timing aspects of the cir¬ cuit of Fig. 2. A system clock 62 provide overall system synchronization and control. An example for the system clock frequency might be 10 MHz. At that frequency, the cycle time is 100 ns, giving a maximum 50 ns on period. The laser pulse duration is controlled by the timer/master counter 50 and laser off counter 52. Preferably, the leading edge of the system clock 62 triggers the genera¬ tion of the laser pulse 64. The trailing edge of the laser pulse is determined by the time set in the laser off counter 52. The waveform 66 of Fig. 3 shows the laser-off counter state, transitioning low when the laser pulse 64 is to terminate. The window open counter pulse 68 runs for a time until the beginning of the data acquisition window 72. The window closed counter pulse 70 runs longer than the window open counter pulse 68, the trailing edge of the window closed counter pulse 70 defining the trail¬ ing edge of the data acquisition window pulse 72. The data acquisition window pulse 72 defines the time period in which the data is supplied from the detector 46
(Fig. 2) to the counter 60. The composite fluorescence signal 74 has an initial steady state portion 76 followed by an intensity decay portion 78. In actuality, for any given single laser pulse, it is more probable than not that no photon will be detected for any data acquisition window. Accordingly, the fluorescence signal 74 would be a compilation of events after numerous laser pulses run with various data acquisition window times.
Fig. 4 shows the detail of the detector PCB 12. Preferably, detection electronics capable of detecting single photon events are used. In the preferred embodi¬ ment, a photomultiplier tube ("PMT") 80 is oriented to detect the fluorescence from a sample (not shown) . Opti¬ mally, the PMT 80 has a low dark current and a high band width, such as 100 MHz. A high voltage power supply 82 supplies power to the PMT 80. A high voltage power supply control signal 84 from the main PCB 14 (shown on Fig. 2) determines the value of high voltage supply from the power supply 82 to the PMT 80. The output of the PMT 80 is amplified as is necessary. Preferably, a comparator 88 allows for selection of the desired pulse amplitude and compensates for offsets in the amplifier 86. The compara¬ tor 88 is preferably controlled by a threshold comparator voltage control (from Fig. 2) . The output of the compara¬ tor 88 goes to the counter 60 (Fig. 2) via gate 58. Pref¬ erably, the cable connection from the main PCB 14 to the detector PCB 12 is a 65 ohm shielded ribbon cable whose length is kept less than 12 inches.
Fig. 5 shows the detail of the laser PCB 10. Laser diode 90 is preferably housed in a beam collimator 92 and mounted directly on laser PCB 10. For convenience, a socket assembly may be used to ease in changing laser diodes 90. Preferably, the collimator assembly 92 and laser diode 90 are further housed within a sealed compart¬ ment 94 with a desiccant (not shown) . Temperature control circuit 96 monitors the temperature of the laser diode 90 via a thermistor 98. A heater 100 is controlled by the temperature control 96 to heat the laser diode 90. The temperature set point control (from Fig. 2) determines the temperature at which the temperature control 96 regulates. By varying the temperature of the laser diode 90, tuning of the diode emission wavelength may be made. Generally, the wavelength shifts 0.3 nanometers per degree centi¬ grade. By varying the temperature, the laser wavelength may be changed to the most advantageous wavelength for the particular fluorescable dye. Ordinarily, the laser is operated from 25° C to 50° C, depending on the particular laser diode and desired wavelength. Optionally, however, the laser may be cooled, using conventional refrigeration techniques. A laser diode driver 102 provides driving power to the laser diode 90. Control inputs to the laser diode driver 102 include the laser on-off control and laser power level set, both of which come from the main PCB 14. Typically, the laser diode 90 is operated at 10 MHz pulse repetition rate and at peak power approximately 6 to 7 times the average rated power output. Exceeding the rated power on a peak basis is possible because the laser pulses are so short that the normal failure mecha- nism, thermal mirror failure, does not occur since the average power is less than the typical continuous operat¬ ing power.
Fig. 6 shows a flow chart for the overall operation. The microprocessor 30 sets the laser on time 104 and laser off time 106. The delay time to the beginning of the data acquisition window is set by the microprocessor 30 and is labeled as start delay 108. Once the data acquisition window opens, pulses exceeding the threshold level as set by the microprocessor 30 are counted at step 110. These events are summed as count 112. If the time for data acquisition has not expired, the decisional block 114 directs the re-initiation of the cycle, causing another laser pulse and counting to begin. When the decision block 114 indicates that the data acquisition time is complete, the results are provided to the computer or other data processing device.
By varying the location of the data acquisition win¬ dow, a histogram of intensity as a function of time may be compiled. Optionally, the data collection and analysis techniques of Dandliker et al. United States Patent No. 4,877,965 are preferably used to further improve the quality of the data.
The timing resolution of the system may be set as precisely as desired. In the preferred embodiment, a timing resolution of 400 picoseconds was selected to permit accurate formation of fluorescent decay times as short as 2 nanoseconds. The data acquisition window is then taken as multiples of the timing resolution value.
Fig. 7 shows a systemwide view of a fluorometer in accordance with this invention designed to determine the time of detection of a photon. After numerous repetitions of the detection cycle, a histogram of the number of events as a function of time is developed. In the pre¬ ferred embodiment, data is collected for time bins, for •example, 1,024 time bins or intervals over 75 nanoseconds results in a bin width of 75 picoseconds. A laser PCB and input optics board 120 generates and directs a laser beam towards a reaction cell 124. Fluorescent light from the reaction cell 124 is detected by the detector PCB 126, whose output is amplified by the amplifier PCB 130, whose signal in turn is supplied to the comparator PCB 132, with the ultimate result being supplied to the data acquisition PCB 128. The result from the data acquisition PCB 128 may be provided to a computer 134 or other functionally simi¬ lar data processing device. Optionally, an interface PCB 136 provides connection between the data acquisition PCB 128 and the laser PCB 120. Further, a thermal control PCB 138 monitors and controls the temperature of the laser diode (not shown) . Additionally, optional filters 140, polarizer 142 , lens 144, and aperture 146 may be used as known to those skilled in the art and described previously in connection with the embodiment described above.
In operation, the laser PCB 120 provides a sequence of laser pulses to the reaction cell 124. The detector PCB 126 detects receipt of photons, if any, and after amplified by amplifier PCB 130, for the signal which exceeds the level set for the comparator PCB 132, an event is considered detected by the data acquisition PCB 128. Broadly speaking, the detection of an event is then used in two ways. First, a running count of the total number of events is made for the time period of interest. In a preferred embodiment, the time period of interest runs continuously during the detection period. Secondly, the detection of an event is used to determine the time at which the event occurred.
Refer to Figs. 8 and 9 for a more detailed under¬ standing of the apparatus and methods utilized herein. The microprocessor 140 and memory 42 operate on the data acquisition PCB 128 to control the system. Preferably, an interface 144, such as an RS 232 port, permits connection with a computer 146 or other data processing or display device. The microprocessor 140 provides numerous control signals, such as: control to the polarizer control 128, the PMT high voltage control, and the ICONT signal, typi¬ cally via digital to analog convertors 150.
An overall clock signal 152 is preferably on the order of 10 MHz. This provides a 100 nanosecond cycle time. The timing circuit 154 generates a laser drive pulse 156 which causes generation of the laser pulse hav¬ ing a shape 160. The timing circuit 154 further causes activation of a delay circuit 156 which in turn, after a predetermined delay, activates ramp generator 158. The ramp voltage 162 begins with a period of delay (see Fig. 9) and then begins a ramp portion. In a preferred embodiment, the delay period is 25 nanoseconds. Upon receipt of a detect event signal 164, the value of the ramp voltage 162 is latched, such as by flip-flop 166. The latched value of voltage from the ramp generator 158 is converted in an analog to digital converter 168 and provided to microprocessor 140 for storage in memory 142. Additionally, the detect event signal 164 is provided to counter 170 which maintains a running count of all detected events.
In the preferred embodiment, the counter 170 counts all events detected, no matter when in the cycle they are detected. Specifically, the counter 170 counts detected events whether during the dark current period, during the laser pulse time, or during the transient state fluores¬ cent decay period. Alternatively, the counter 170 may be activated only during desired times, for example, being inactivated during the dark current time.
In operation, when a detected event 164 is received by the data acquisition PCB 128 (Fig. 8) , a certain amount of time is required to determine the time of the detected event, process it, and store it. While this process is ongoing, the time detection system ignores new photons or events until the previously received photon time has been completed. Depending upon the particular hardware chosen, the time during which new photons are ignored can be on the order of 30 microseconds. If the clock frequency is 10 MHz, approximately 300 laser pulses are ignored. Gen¬ erally, this is insignificant in all but the highest con¬ centration of fluorophores. At nominal concentrations, typical input rates of photon events from the PMT is approximately 10,000 per second. Accordingly, a photon is detected roughly every 1,000 pulses. For higher concen¬ tration of fluorophore, pulse rates may increase by orders of magnitude. To maintain linearity, laser diode peak power may be lowered or apertures may be placed in the detection path. Alternatively, for larger pulse rates, the counter 170 monitors all detected events, independent of the timing of the detected event.
Through this method, the shape of the histogram may be determined by measuring the time of the detected event for a large number of samples. However, because certain events may be ignored during the processing time, the counter 170 provides for the calculation of a scale factor so as to provide a true measure of the intensity of the fluorophore decay as a function of time. In the preferred method, the dark current signal level (the level of cur¬ rent or detected events existing even with no laser pulse or fluorescent decay) is detected. Next, the value of the dark current is subtracted from the total number of counts in each bin. In this way, a true measure of the number of detected events occurring during that time bin is set. Next, the total number of counts in the time bins are summed, giving a measure of the total number of events detected. Next, the ratio of events counted by counter 170 and the number of events found by integrating all of the bin counts (less the dark current) is multiplied times the value in each bin. In this way, compensation is made for events which occurred during the analysis, as indi¬ cated by a detected event stored by counter 170, but which did not form part of the histogram as detected by the sampling of values from the ramp voltage 162 (presumably because an event was being processed) .
It is necessary to give equal weight to detection of events for all time bins. If the system were to always record the first detected event after the laser pulse, for example, a disproportionate number of events would be detected early in the histogram, thereby skewing the histogram results. One method for avoiding such skew in the histogram is to provide for a random starting time for detection. In the preferred embodiment, this time is determined by re-enabling the ability to measure the ramp voltage 160 to any time directly following storage of the preceding event. In this way, no down time is suffered, and, given the relatively long period of time for data acquisition and storage, the exact time of resumption of monitoring for a subsequent detected event is essentially random.
A detailed block diagram for the laser PCB 120 is provided in Fig. 10. The laser PCB 120 takes the laser drive pulse 158 from the data acquisition processor board
(Fig. 8) and generates a laser light pulse. In a pre- ferred embodiment, the duration of the pulse is on the order of a few nanoseconds, and is of relatively high power. An incoming rising edge in the laser drive pulse 158 causes generation of a laser flash. Input logic 170, 174, and 176 generate a very sharp rising edge, which is supplied to the high-powered digital driver 178. The digital driver 178 provides power to the laser diode 180. The current used by the laser diode 180 is set by the signal ICONT from the data acquisition PCB (Fig. 8) . The duration of the laser pulse may be varied by changing the delay 172. Further, the amplitude of the laser pulse is varied by setting the current value ICONT. A reference diode 182 monitors the long term stability of the laser output. Preferably, the reference diode 182 is located downstream of the optics and filter through which the laser beam passes. In this way, the total input power directed to the sample may be monitored. Various factors which affect total input power would include laser perfor¬ mance or degradation, cleanliness of the optical compo¬ nents or degradation of the laser filter. A photocurrent monitor 184 monitors the photocurrent of the laser diode 180. Since the pulse length and repetition rate are known, the average power being generated by the laser diode 180 may be calculated. This power reading, labeled VMON, is fed back to the data acquisition PCB (Fig. 8) .
Additionally, an optional heater 186 and thermistor and temperature control 188 provide temperature control to the laser diode 180. The temperature set point is provid¬ ed from the data acquisition PCB to the heater 186 and control 188. As described in connection with the first embodiment, varying the temperature changes the wavelength of the laser diode 180. The detector PCB 126 is described in detail in Fig. 11. The photomultiplier tube 190 receives fluores¬ cent radiation from the sample. A high voltage generator 192, under control the PMT high voltage control signal 194 as amplified 196 provides high voltage to the PMT 190. The output of the PMT 190 is passed through amplifier 192 and sent through comparator 194. If the detected and amplified value exceeds the reference value, the compara¬ tor passes the signal as output to the data acquisition PCB. Preferably, the amplifier 192 is connected to the comparator 194 by dual coaxial cable providing a differen¬ tial signal. The comparator 194 is similarly connected via coaxial cables to the data acquisition PCB. Fig. 12 shows a flow chart for the preferred method of operation. During the initialization phase 200, the following items are set: the PMT voltage, laser intensi¬ ty, data acquisition time, liquid crystal polarizer ("LCP") cycles, and LCP to parallel. Next, data acquisi¬ tion starts 202. After the laser pulse 204 and a delay 206, the ramp 208 begins. If a photon is detected 210, the ramp voltage is frozen 212 and the height measured and converted to digital 214. The data updates,216 the appro- priate bin. If the data acquisition time decision 218 exceeds the allowed time, the hardware counter is stopped. If data acquisition time remains, the laser pulse sequence is begun again. When data acquisition time is completed, the data from the counter is stored 220. Optionally, the polarizer may be changed to the other orientation instead 222.
EXPERIMENTAL RESULTS
The devices and methods described herein have been utilized with fluorescence measurements from numerous sys- terns, especially biological systems. The data reported herein were generated with the time of detection system.
The fluorometry system described herein when used in conjunction with the fluorescable dyes described in copending applications to Arrhenius and Dandliker and Hsu result in an improvement in signal detection of over 100 times over conventional techniques. The following table lists the detectable concentration level of dye at the point where the intensity of the desired signal equals the intensity of the background. The buffer used contains 1% bovine serum albumin. The data are as follows:
Figure imgf000023_0001
By selecting a dye with a longer wavelength and by utilizing time gating and the time of detection techniques described above, a significant improvement in the detected signal intensity is achieved. As to linearity, Fig. 13 shows a log-log plot of the intensity as a function of Digoxin probe concentration. The results show the system to be linear over four orders of magnitude. Further, concentrations as low as approxi¬ mately IO"13 moles per liter may be detected. An accurate system should have such a linear response, since as the concentration of fluorescable material decreases, there should be a correspondingly linear decrease in the number of counts detected.
Actual data from a sample is shown in Fig. 14. The intensity (number of counts per 10 seconds) is shown on the y-axis measured in thousands. The x-axis shows the time bin number, with each bin corresponding to a 75 pico¬ second interval. The scatter curve peaks slightly to the left of the peak of the fluorescence curve. The dark current counts are shown generally in the time from bin number 200 to bin number approximately 300. The decay of the fluorescence curve as a function of time provides a histogram which may be used in conjunction with data analysis techniques such as those disclosed in Dandliker et al. U.S. Patent No. 4,877,965.
As described in detail above, the time of detection system forms a histogram which accurately depicts the shape of the intensity curve, and then scales that shape to provide an absolute measure of intensity as a function of time. In the preferred embodiment, the method used is to monitor the total number of counts with a high speed hardware counter and to determine the total number of counts comprising the shape histogram by integrating those counts. The histogram shape curve is then multiplied by the ratio of the hardware counts to the total integrated counts. Fig. 15 shows the integrated timing system counts as a function of high speed counter counts. A maximum of 33,000 counts per second may be detected by the timing system counter. This however is a function of the speci¬ fic hardware chosen. If a dedicated processor or faster processor were chosen, as are design choices available to those skilled in the art, the time required to store a time of receipt of an event is decreased, and accordingly, the number of counts per second may be increased.
Fig. 16 shows the intensity (in millions) as a func¬ tion of probe concentration (in moles per liter x 1010) for two curves. The upper curve shows the normalized counts and the lower curve shows the raw counts. Through u . ■ of the techniques described above, the raw counts may be in¬ verted into normalized counts, thereby providing liner . y of intensity as a function of probe co.-. entraci n. In the time of rec: ;pt system, ..ιe high repetition rates of the laser di, .2 combined with the hardware counter compensation have provided the best useful data. Preferably, the photon flux is relatively low. With a relatively low photon flux, the probability of two photons hitting the PMT at the same time is substantially reduced, thereby avoiding system non-linearity. As the concentra¬ tion of the fluorophore is decreased, the laser power and/or repetition rate may be increased to speed data acquisition. Fig. 17 shows a graph of transient-state polarization versus digoxin concentration.
A 20 microliter sample containing known levels of digoxin were incubated with 25 microliters of rabbit anti- digoxin antibody for 5 minutes in 100 microliter of buf- fer. The 20 microliters of fluorescently labelled digoxin probe (at a concentration 5 x 10"11M was then added and incubated for an additional 5 minutes. Finally, the solu¬ tions were diluted with 1 milliliter of buffer. The fluorescence signal was then read using the time of detec- tion hardware apparatus.
Though the invention has been described with respect to a specific preferred embodiment, many variations and modifications will immediately become apparent to those skilled in the art. It is therefore the intention that the appended claims be interpreted as broadly as possible in view of the prior art to include all such variations and modifications.

Claims

We claim:
1. A fluorometer for exciting a sample including a fluorophore and for detecting fluorescent emissions from the sample comprising: a laser diode for exciting the sample, a detector positioned to receive fluorescent emission, and means for determining the time of receipt of the fluorescent emission, said means including a ramp generator.
2. The fluorometer of Claim 1 wherein the means for determining the time of receipt of the fluorescent emis¬ sion further includes a means to sample the ramp.
3. The fluorometer of Claim 1 further including a counter operatively connected to receive the output of the detector.
4. A method for obtaining improved fluorescence signals from a background in a transient state fluorometry system employing the steps of exciting a fluorophore with a pulse of radiation, and then detecting the decay fluor¬ escence and background as a function of time and as a function of polarization, the improvement including adding the step of ignoring the decay fluorescence and background occurring during and immediately after the pulse of radiation.
5. The method of Claim 4 wherein the step of ignor¬ ing the decay fluorescence and background includes the step of time gating to exclude the decay fluorescence and background immediately after the pulse of radiation.
6. The method of Claim 4 wherein the step of ignor¬ ing the decay fluorescence and background includes obtain- ing, but not using, the decay fluorescence and background occurring immediately after the pulse of radiation.
7. A method for generating a histogram of the intensity as a function of time for a transient state fluorescence determination comprising the steps of: detecting events of fluorescence, counting the total number of detected events, determining a preliminary histogram of shape of the histogram, counting the number of events comprising the preliminary histogram, and multiplying the preliminary histogram times the ratio of the count of the total number of events and the count of the number of events comprising the pre- liminary histogram.
8. The method of Claim 7 further including the step of measuring the dark current and subtracting the dark current contribution from the preliminary histogram prior to the counting and multiplication steps.
9. The method for generating a histogram of detected events in a transient state fluorometry system comprising the steps of: a) monitoring for a detected event, b) upon an event, determining the time of occurrence of the detected event, c) storing the time determined in step b and ignoring for purposes of step b other detected events while performing this step, d) upon completion of step c, resume monitoring at step a at a time after completion of step c, and e) generating a histogram using the times stored in step c.
10. The method of Claim 9 wherein in step d, the monitoring at step a is measured immediately after comple¬ tion of step c.
11. The method of Claim 9 wherein in step b, the determination of the occurrence of the time of an event is done by sampling a ramp voltage.
12. The method of Claim 11 wherein after the ramp voltage is sampled, the voltage is converted to a digital representation.
13. The method of Claim 9 wherein the time after completion of step c is a random time.
14. A fluorometry system comprising: a laser capable of being pulsed at greater than 10,000 cycles per second, a holder adapted to receive a sample including a caged dicarboxy silicon phthocyanine dye, and a detector positioned to receive fluorescent emission from the dye.
15. The fluorometry system of claim 14 wherein the laser is a laser diode.
16. The fluorometry system of claim 14 further including means for determining the time of receipt of the fluorescent emission.
17. The fluorometry system of claim 14 further including a time gate generator.
18. The fluorometry system of claim 14 wherein the dye is a caged dicarboxy silicon phthocyanine-digoxigenin.
19. A fluorometer for exciting a sample including fluorophore and for detecting fluorescent emissions from the sample comprising: a laser diode for exciting the sample, a detector position to receive fluorescent emission, means for determining the time of receipt of the fluorescent emission, and a counter operatively connected to receive the output of the detector.
20. The fluorometry system of claim 19 further including a time gate generator.
21. The fluorometry system of claim 20 wherein the time gate generator gates the output of the detector.
22. The fluorometry system of claim 20 which further includes a gate which receives as input the output of the detector and is controlled by the output of the time gate generator.
23. The fluorometry system of claim 20 wherein the time gate generator includes a counter.
24. The fluorometry system of claim 23 wherein the time gate generator includes a window open counter and a window closed counter.
25. The fluorometry system of claim 19 wherein the detector is a photomultiplier tube.
26. The fluorometer of claim 19 wherein the detector is red sensitive.
27. The fluorometer of claim 19 wherein the detector is infrared sensitive.
28. The fluorometer of claim 19 wherein the laser diode is rotatable relative to the sample.
29. The fluorometer of claim 19 wherein the laser diode radiates in the red to infrared range.
30. The fluorometer of claim 19 wherein the laser diode has a variable wavelength.
31. The fluorometer of claim 30 further including a temperature variation device.
32. The fluorometer of claim 30 wherein the laser diode is a turnable laser diode.
33. The fluorometer of claim 32 wherein the laser diode is a quantum well laser diode.
34. The fluorometer of claim 19 further including optics.
35. The fluorometer of claim 19 further including a display.
36. A fluorometer for exciting a sample including a fluorophore and for detecting fluorescent emissions from the sample comprising: a laser diode for exciting the sample, a detector positioned to receive fluorescent emis¬ sion, and means for determining the time of receipt of the fluorescent emission, said means including a delay genera- tor.
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Cited By (9)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
EP0702226A3 (en) * 1994-09-19 1996-06-26 Hamamatsu Photonics Kk Decay characteristic measuring apparatus
WO1998009154A1 (en) * 1996-08-29 1998-03-05 Boehringer Mannheim Gmbh System for distinguishing fluorescent molecule groups by time resolved fluorescence measurement
DE19702914A1 (en) * 1997-01-28 1998-09-17 Max Planck Gesellschaft Method of determining predetermined properties of target particles in sample medium
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US6690463B2 (en) 2000-02-10 2004-02-10 Evotec Biosystems Ag Fluorescence intensity and lifetime distribution analysis
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Families Citing this family (48)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US6060598A (en) * 1990-05-15 2000-05-09 Hyperion, Inc. Fluorescence immunoassays using fluorescent dyes free of aggregation and serum binding
US5426306A (en) * 1993-10-21 1995-06-20 Associated Universities, Inc. Fast repetition rate (FRR) fluorometer and method for measuring fluorescence and photosynthetic parameters
US5919140A (en) 1995-02-21 1999-07-06 Massachusetts Institute Of Technology Optical imaging using time gated scattered light
EP1760151B1 (en) * 1996-11-20 2012-03-21 Crucell Holland B.V. Adenovirus compositions obtainable by an improved production and purification method
US5994707A (en) * 1997-03-18 1999-11-30 Physical Optics Corporation Modular fiber optic fluorometer and method of use thereof
US6071748A (en) * 1997-07-16 2000-06-06 Ljl Biosystems, Inc. Light detection device
US6097025A (en) * 1997-10-31 2000-08-01 Ljl Biosystems, Inc. Light detection device having an optical-path switching mechanism
US6469311B1 (en) 1997-07-16 2002-10-22 Molecular Devices Corporation Detection device for light transmitted from a sensed volume
US6326605B1 (en) 1998-02-20 2001-12-04 Ljl Biosystems, Inc. Broad range light detection system
US6297018B1 (en) 1998-04-17 2001-10-02 Ljl Biosystems, Inc. Methods and apparatus for detecting nucleic acid polymorphisms
US6825921B1 (en) 1999-11-10 2004-11-30 Molecular Devices Corporation Multi-mode light detection system
WO2000050877A1 (en) 1999-02-23 2000-08-31 Ljl Biosystems, Inc. Frequency-domain light detection device
WO2000006991A2 (en) 1998-07-27 2000-02-10 Ljl Biosystems, Inc. Apparatus and methods for spectroscopic measurements
US6576476B1 (en) 1998-09-02 2003-06-10 Ljl Biosystems, Inc. Chemiluminescence detection method and device
US6992761B2 (en) * 1997-09-20 2006-01-31 Molecular Devices Corporation Broad range light detection system
US6121053A (en) * 1997-12-10 2000-09-19 Brookhaven Science Associates Multiple protocol fluorometer and method
US6055451A (en) 1997-12-12 2000-04-25 Spectrx, Inc. Apparatus and method for determining tissue characteristics
AU2775899A (en) * 1998-02-20 1999-09-06 Ljl Biosystems, Inc. Broad range light detection system
AU5667599A (en) 1998-07-27 2000-02-21 Ljl Biosystems, Inc. Apparatus and methods for time-resolved spectroscopic measurements
CA2343401C (en) * 1998-09-11 2009-01-27 Spectrx, Inc. Multi-modal optical tissue diagnostic system
JP2001078175A (en) 1999-07-07 2001-03-23 Fuji Photo Film Co Ltd Fluorescent observation device
JP2001070227A (en) 1999-07-07 2001-03-21 Fuji Photo Film Co Ltd Fluorescent observing device
US6402986B1 (en) 1999-07-16 2002-06-11 The Trustees Of Boston University Compositions and methods for luminescence lifetime comparison
US6447995B1 (en) 2000-10-04 2002-09-10 Genvec, Inc. Utilizing intrinsic fluorescence to detect adenovirus
ATE403142T1 (en) * 2000-12-21 2008-08-15 Evotec Ag METHOD FOR CHARACTERIZING SAMPLES OF SECONDARY LIGHT EMITTING PARTICLES
US20030136921A1 (en) * 2002-01-23 2003-07-24 Reel Richard T Methods for fluorescence detection that minimizes undesirable background fluorescence
JP4074136B2 (en) * 2002-05-29 2008-04-09 浜松ホトニクス株式会社 Fluorescence lifetime distribution image measuring apparatus and measuring method thereof
US20030224354A1 (en) * 2002-05-30 2003-12-04 Introgen Therapeutics Inc. Quantifying viral particles with intrinsic fluorescence
US7371524B2 (en) * 2003-06-17 2008-05-13 Hannjorg Hereth Substituted azaporphyrins as fluorescence labels
CA2584186A1 (en) * 2004-10-18 2006-08-31 Macquarie University Fluorescence detection
US7391512B2 (en) * 2004-12-22 2008-06-24 Avago Technologies General Ip Pte. Ltd. Integrated optoelectronic system for measuring fluorescence or luminescence emission decay
JP4652868B2 (en) * 2005-03-30 2011-03-16 独立行政法人産業技術総合研究所 Fluorescence analysis method
US7839500B2 (en) * 2005-05-30 2010-11-23 Jerker Widengren Apparatus, method and computer program for spectroscopic measurements and analysis
DE102005027896B4 (en) 2005-06-16 2012-03-15 MAX-PLANCK-Gesellschaft zur Förderung der Wissenschaften e.V. Method for optically measuring a sample
US8232091B2 (en) 2006-05-17 2012-07-31 California Institute Of Technology Thermal cycling system
DE102006048346A1 (en) * 2006-10-12 2008-04-17 Eppendorf Ag Method for the device for the quantitative real-time analysis of fluorescent samples
KR100885927B1 (en) * 2007-10-16 2009-02-26 광주과학기술원 Apparatus and method for measuring fluorescence lifetime
WO2009089315A1 (en) * 2008-01-08 2009-07-16 Kinase Scientific, Llc Method to detect hemolytic streptococcus and optoelectronically determine results
DE102008018475A1 (en) 2008-04-11 2009-10-15 Carl Zeiss Ag Apparatus and method for luminescence measurement
US8104512B2 (en) * 2008-09-25 2012-01-31 Masco Corporation Of Indiana Spout tip retention method
WO2010115160A2 (en) * 2009-04-03 2010-10-07 Helixis, Inc. Devices and methods for heating biological samples
EP2301666B1 (en) * 2009-09-09 2021-06-30 Cole-Parmer Ltd. Optical system for multiple reactions
US9222850B2 (en) * 2013-03-14 2015-12-29 Axonoptics, Llc Integrated optics reflectometer
US9557243B2 (en) 2012-03-14 2017-01-31 Axonoptics Llc Integrated optics reflectometer
DE102012113024A1 (en) * 2012-12-21 2014-06-26 Hamilton Bonaduz Ag Optical measuring device
US9140648B2 (en) 2013-03-12 2015-09-22 Ecolab Usa Inc. Fluorometer with multiple detection channels
US8970724B2 (en) * 2013-03-15 2015-03-03 National Security Technologies, Llc Mach-zehnder based optical marker/comb generator for streak camera calibration
RU2751176C1 (en) * 2020-12-28 2021-07-09 Акционерное общество "Специальное конструкторско-технологическое бюро Кольцова" Multi-position switching device

Citations (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US4198587A (en) * 1977-11-15 1980-04-15 U.S. Philips Corporation Color CRT shielding cone having four metal plates extending from corners of smaller aperture to wall coating
US4855930A (en) * 1987-03-27 1989-08-08 Chimerix Corporation Method and appartatus for improved time-resolved fluorescence spectroscopy
US4877965A (en) * 1985-07-01 1989-10-31 Diatron Corporation Fluorometer
US5071249A (en) * 1988-10-05 1991-12-10 Hamamatsu Photonics K.K. Light waveform measuring apparatus
US5196709A (en) * 1991-05-03 1993-03-23 University Of Maryland Systems Fluorometry method and apparatus using a semiconductor laser diode as a light source

Family Cites Families (6)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US4058732A (en) * 1975-06-30 1977-11-15 Analytical Radiation Corporation Method and apparatus for improved analytical fluorescent spectroscopy
US4198567A (en) * 1977-10-25 1980-04-15 Peter Eneroth Method and apparatus for discrimination between scattered excitation radiation and low level fast decaying fluorescent radiation
US4895156A (en) * 1986-07-02 1990-01-23 Schulze John E Sensor system using fluorometric decay measurements
US4716363A (en) * 1987-05-08 1987-12-29 Hewlett-Packard Company Exponential decay time constant measurement using frequency of offset phase-locked loop: system and method
US4857735A (en) * 1987-10-23 1989-08-15 Noller Hans G Light emitting diode spectrophotometer
US5151869A (en) * 1990-02-16 1992-09-29 The Boc Group, Inc. Frequency domain fluorometry using coherent sampling

Patent Citations (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US4198587A (en) * 1977-11-15 1980-04-15 U.S. Philips Corporation Color CRT shielding cone having four metal plates extending from corners of smaller aperture to wall coating
US4877965A (en) * 1985-07-01 1989-10-31 Diatron Corporation Fluorometer
US4855930A (en) * 1987-03-27 1989-08-08 Chimerix Corporation Method and appartatus for improved time-resolved fluorescence spectroscopy
US5071249A (en) * 1988-10-05 1991-12-10 Hamamatsu Photonics K.K. Light waveform measuring apparatus
US5196709A (en) * 1991-05-03 1993-03-23 University Of Maryland Systems Fluorometry method and apparatus using a semiconductor laser diode as a light source

Non-Patent Citations (2)

* Cited by examiner, † Cited by third party
Title
Die Angewandte Makromolekulare Chemie, 1978, MEYER et al., "Polymer mit dem Zentralatom eines Makrocyclus in der Hauptkette", Vol. 72, pp. 173-184 and Chem. Ab. 90 (14),90:10438H, p. 1, April 2, 1979, see Abstract. *
Die Makromolekulare Chemie, Vol. 176, 1975, HARTMANN et al., "Polymere mit dem Zentralatom in der Hauptkette, 2", pp. 831-847 and Chem. Ab., Vol. 83, p. 4, No. 79670p, see Abstract. *

Cited By (12)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
EP0702226A3 (en) * 1994-09-19 1996-06-26 Hamamatsu Photonics Kk Decay characteristic measuring apparatus
WO1998009154A1 (en) * 1996-08-29 1998-03-05 Boehringer Mannheim Gmbh System for distinguishing fluorescent molecule groups by time resolved fluorescence measurement
DE19702914A1 (en) * 1997-01-28 1998-09-17 Max Planck Gesellschaft Method of determining predetermined properties of target particles in sample medium
DE19702914C2 (en) * 1997-01-28 1998-12-24 Max Planck Gesellschaft Method and arrangement for determining predetermined properties of target particles of a sample medium
DE19718016A1 (en) * 1997-04-29 1998-11-05 Drexhage Karl Heinz Method for the optical detection of analyte molecules in a natural biological medium
GB2330904A (en) * 1997-10-29 1999-05-05 Lab Molecular Biophotonics Fluorescence lifetime measurement system
US5990484A (en) * 1997-10-29 1999-11-23 Laboratory Of Molecular Biophotonics Method and apparatus for measuring fluorescence
US6690463B2 (en) 2000-02-10 2004-02-10 Evotec Biosystems Ag Fluorescence intensity and lifetime distribution analysis
WO2004031748A1 (en) * 2002-10-01 2004-04-15 Hamamatsu Photonics K.K. Fluorescence measuring device
EP2418532A1 (en) * 2010-08-13 2012-02-15 Leica Microsystems CMS GmbH Method for separating detection signals in the beam of an optical device
US9651765B2 (en) 2010-08-13 2017-05-16 Leica Microsystems Cms Gmbh Method for separating detection signals in the beam path of an optical device
WO2022152777A1 (en) * 2021-01-15 2022-07-21 F. Hoffmann-La Roche Ag Storage stable caged haptens

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