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LUMINESENCE
The term 'luminescence' was introduced in 1888 by
  Eilhard Wiedemann .
“Luminescence is the emission of light by a
  substance. It occurs when an electron returns
  to the electronic ground state from an excited
  state and loses it's excess energy as a photon.”
Luminescence spectroscopy is a collective name
  given to three related spectroscopic techniques.
  They are;
   Molecular fluorescence spectroscopy
   Molecular phosphorescence spectroscopy
   Chemiluminescence spectroscopy
TYPES OF LUMINESENCE
 Bioluminescence
 Chemiluminescence
       Electrochemiluminescence
 Crystalloluminescence
 Electroluminescence
 Mechanoluminescence
     Triboluminescence
     Fractoluminescence
     Piezoluminescence
 Radioluminescence
 Sonoluminescence
 Thermoluminescence
PHOTOLUMINESENCE
   “Photoluminescence (PL) is the spontaneous
   emission of light from a material under optical
   excitation.”
It is futher subdivided into two types
  a. Flourescence
  b. Phosphorescence
ACTIVATION AND DEACTIVATION IN
PHOSPHORESENCE
 The absorption of a photon of suitable energy
  causes the molecule to get excited from the ground
  state to one of the excited states. This process is
  called as excitation or activation and is governed
  by Franck-Condon principle.
 According to this principle, the electronic transition
  takes place so fast (~10-15 s) that the molecule
  does not get an opportunity to execute a vibration,
       i.e., when the electrons are excited the internuclear
        distance does not change.
•   The basis for the principle is that the nuclei are
    very massive as compared to the electrons and
    therefore move very slowly.
•   At the ground state , the molecular orbitals are occupied
    by two electrons. the spins of the two electrons in the
    same orbital must be antiparallel. This implies that the
    total spin, S, of the molecule in the ground state is
    zero [½ + ( ½)].
•   This energy state is called “singlet state” and is labeled
    as S0.
•   The electron spins in the excited state achieved by
    absorption of radiation may either be parallel or
    antiparallel. Accordingly, this may be a triplet (parallel)
    or a singlet (antiparallel) state.
   The deactivation processes can be broadly categorized
    into two groups given below.
      • Nonradiative deactivation
            Vibrational Relaxation
            Internal Conversion
             Intersystem Crossing
      • Radiative deactivation
          Fluorescence
          Phosphorescence
JABLONSKI DIAGRAM
DIFFERENCE BETWEEN PHOSPHORESCENCE
AND FLUORESCENCE

Phosphorescence                      Fluorescence

 The emission could           The emission could
  proceed either from a         proceed only from a
  singlet or triplet state.     singlet state.
 short-live electrons         longer lifetime of the
  (<10-5 s) in the excited      excited state (second
  state of fluorescence         to minutes)
FLUORESCENCE AND
PHOSPHORESCENCE
   Fluorescence      Phosphorescence
PHOSPHORESCENCE SPECTROSCOPY
Phosphorescence Spectroscopy is the
 spectroscopic study of the radiation
 emitted by the lifetime of
 phosphorescence.
Phosphorescence has been observed
 from a wide variety of compounds and is
 differentiated from fluorescence by the
 long-lived emission of light after
 extinction of the excitation source. The
 first analytical uses of phosphorescence
 were published in 1957 by Kiers et. al.
FIG:SRAL2O4 ,PIGMENTS IN THE DARK AND THAN PIGMENTS IN
THE DARK AFTER 4 MIN
PHOSPHORIMETRY
   Spectrophosphorimeter        is  similar   to   a
    Spectrofluorimeter except that the former
    instrument must be fitted with
     1) a sample system which is maintained at liquid
    nitrogen temperature
    2) A Rotating-shutter device commonly called a
    phosphoroscope and
    .
SAMPLE PREPARATION
   The majority of phosphorescence measurements are carried out in
    rigid media at the temperature of liquid nitrogen
   The criteria for solvent selection are:
      good solubility of the analyte
      formation of a clear rigid glass at 77 K
      low phosphorescence background (high purity)
   For polar compounds, ethanol is an excellent solvent and small
    For non-polar compounds, the most popular solvent is a mixture of
    diethyl ether, isopentane and ethanol in the ratio of 5:5:2 respectively
   The samples are placed in a narrow quartz tube(internal diameter
    varying from 1 to 3 mm).
   The dimensions are a compromise between too small a diameter
    and too large a diameter.
   The sample tubes are placed in liquid nitrogen held in a quartz
    Dewar flask, and the latter placed in the sample holder known as a
    phosphoroscope.
Phosphorescence can also be observed from
  solid samples at room temperature, and the
  compounds can be divided into two types.
 The first includes inorganic salts and oxides such
  as the rare earths, europium and uranium
 The second type of compounds are those which
  exhibit phosphorescence when absorbed onto
  certain substrates such as
  paper, cellulose, silica, etc.
    Polar organic molecules, when absorbed onto
     filter paper from solutions containing 1 N
     NaOH and thoroughly dried, exhibit
     phosphorescence.
 Studies have shown that the phosphorescence
  could be enhanced by the addition of heavy
  atoms, for example iodine, silver, lead
PHOSPHOROSCOPE
INSTRUMENTATION
 Excitation Source
 Filters/Monochromators for excitation radiations

 Phosphorscope(sample Cell)

 Filters and Monochromators for emission

 Detectors
EXCITATION SOURCE
   High intensity source of UV light are used
       Lasers – A laser makes it possible to have narrow wavelength intervals
        that offer very high energy irradiation. This is useful when a large amount
        of energy is needed to produce the Phosphorescence in the sample.

       Photodiodes – Photodiodes are specialized diodes that can be
        configured in a manner that allows electrons to flow towards the sample
        so that the excess energy excites the phosphorescent particles.

       Xenon Arcs – Arcs of Xenon can produce the right amount of radiation for
        Phosphorescent materials.

       Mercury Vapor – Since mercury vapor can create ultraviolet radiation
        when electrical current is passed through it, it is good for use with
        materials that shows Phosphorescence under the ultraviolet radiation.
Care should be taken as Intense UV light is hazardous for health
 Filters and monochromators used in a
  phosphorimeter device.
 Filters
   Absorption
   Interfernce
 Monochromators     allow wavelength adjustment.
  Monochromators make it possible to do so with a
  diffraction grating.
     The primary filters that excite the sample provide the appropriate wavelength
      while the secondary filters monochromate the emitted light when sent to the
      detector.
 Phosphoresence              spectroscopy detectors may have
  a
     single channel (single wavelength from sample)
      or multiple channels (multiple wavelengths detection)
PHOSPHOROSCOPE
1.The Becquerel or rotating disc phosphoroscope
 A rotating disk excitation optical chopper, with three open
  and three larger opaque areas, is used to alternately
  excite the sample and allow phosphorescence to be
  measured.
 By measuring the phosphorescence intensity at several
  time intervals along the emission decay curve, a recorder
  trace of the decay with respect to time can be produced.
 The analytical precision and accuracy for quantitative
  measurements is improved by rotating the sample tube.
  This minimizes variation in the signal due to sample
  inhomogeniety resulting from imperfect glass formation at
  lowtemperatures .
2.The Rotating-Can Phosphoroscope:
      It consists of hollow cylinder having one or more slit which are
       equally spaced in the circumference.
      This is rotated by a variable-speed motor(>1000rpm)
      when the rotating-can is rotated by a motor the sample is excited
       show fluorescence and phosphorescence
   For Fluorescence The emission monochromator is blocked by the
    can so that fluorescence and scattered radiation cannot be detected.
   As the can rotates, the excitation beam is blocked and the
    fluorescence and scattered radiation decay to a negligible amount.
    Further rotation of the can will bring the window into alignment with
    the emission monochromator entrance slit and phosphorescence
    radiation will pass into the emission monochromator and onto the
    sample photomultiplier
PULSED SOURCE-TIME
RESOLVED PHOSPHORIMETRY
   was first proposed by Fisher and Winefordner in 1972.
   A pulsed source produces higher peak intensities than a
    continuously operated xenon lamp resulting in a greater peak
    phosphorescence emission intensity.
   Pulsed source phosphorimetry has the advantage of time
    resolution compared with a mechanically modulated system
    permitting the analysis of organic phosphor with short lifetimes
    (0.1 to 50 microsec)
   The xenon lamp produces a burst of energy with a width a half
    peak intensity of less than 10 μsec.
   The signals from the sample photomultiplier are gated and
    both the
    delay of the start of the gate after the start the flash
    Timing is performed by a crystal clock and is highly accurate.
   a quantum-corrected reference photomultiplier is used to
    monitor the flash intensity and the signals from th sample and
    reference
FIG:SCHEMATIC DRAWING OF GATED
PHOSPHORIMETER SETUP.
THE PERKIN ELMER LS 55 LUMINESCENCE
SPECTROMETER
   It is a very versatile
    instrument that allows
    measurement of
    fluorescence,
    phosphorescence ,
    chemiluminescence and
    bioluminescence of a liquid,
    solid, powder, or thin film
    sample
    Fluorescence data are
    collected at the instant of the
    flash while
    phosphorescence data are
    collected in the dark period
    between each flash.
APPLICATIONS OF PHOSPHORESCENCE
SPECTROSCOPY

 Pharmaceutical     Applications
 Clinical   Applications

 Environmental     Applications

 Forensic    Applications

 Entertainment    Applications
PHARMACEUTICAL APPLICATIONS
 The majority of phosphorescence applications have
  been applied in the drug and pharmaceutical field
  and in the analysis of pesticides
 A number of the sulphonamide class of drugs
  exhibit phosphorescence as do
  phenobarbital, cocaine, procaine, chlorpromazin
  and salicylic acid.
CLINICAL APPLICATIONS
 The phosphorescence intensity of the rare earths
  increases tremendously when they are covalently
  bound to certain molecules and this feature has
  been used in the analysis of transferin in blood
 dual-wavelength phosphorimeter used to measure
  microvascular PO2 (µPO2) in different depths in
  tissue and demonstrates its use in rat kidney.
Entertainment Applications
 use of phosphor coated stamps and envelopes has
  appeared which gives a fascinating insight into the
  practical use of phosphorescence
 The rare earths and uranyl elements phosphoresce and a
  number of them, particularly europium and terbium, are
  used as phosphors in lamps and TV tubes.
ENVIRONMENTAL APPLICATIONS
 Phosphorescence has been used in the detection
  of air and water-borne pollutants
 for the analysis of impurities in polycyclic aromatic
  hydrocarbons and in petroleum products .
CONCLUSION
 Although the applications of phosphorescence have
 been somewhat limited in the past, the introduction
 of new instrumentation and advances made in room
 temperature phosphorescence have lead to an
 increase in its use, particularly in clinical chemistry ,
 the forensic, environmental and pharmaceutical
 fields.
REFERENCES
1.Kiers, R.J., Britt, R.D., Wentworth, W.E., Anal. Chem., 29, 202
   (1957).
2. Fluorescence Detection in Liquid Chromatography., Rhys
   Williams, A.T., PerkinElmer Limited (1980).
3. Schulman, E. M., Walling, C., J. Phys. Chem., 77, 902 (1973).
4. Hollifield, H. C., Winefordner, J. D., Anal. Chem., 40, 1759
   (1968).
5. Zweidinger, R., Winefordner, J. D., Anal. Chem., 42, 639 (1970).
6. Fisher, R. P., Winefordner, J. D., Anal. Chem., 44, 948 (1972).
7. Harbaugh, K.F., O’Donnell, C. M., Winefordner, J. D., Anal.
   Chem., 45, 381 (1973.)
8. Sawicki, E., Pjaff, J. D., Anal. Chim. Acta., 32, 521 (1965).
9. Giffard, L. A., Miller, J. N., Burns, D. T., Bridges, J. W., J.
   Chromatog., 103, 15(1975).
10. de Lima, C. G., Nichola, E. M., Anal.Chem., 50, 1658 (1978).
11. O’Donnell, C. M., Winefordner, J. D., Clin. Chem., 21, 285
   (1975).
12. Aaron, J. J., Winefordner, J. D., Anal.Chem., 44, 2127
  (1972).
13. Vo. Dinh, T. Winefordner, J. D., Appl. Spec. Rev., 13, 261
  (1977).
14. Saunders, L. B., Winefordner, J. D., Talanta, 16 407 (1969).
15. Aaron, J. J. Winefordner, J. D., Anal. Chem., 19, 21 (1972)
16. Hollifield, H. C., Winefordner, J. D., Talanta, 12, 860 (1965).
17. Winefordner, J. D., Latz, H. W., Anal. Chem., 35, 1517
  (1963).
18. Perry, A. W., Winefordner, J. D., Anal. Chem., 43, 781
  (1971).
19. Aaron, J. J., Kaleel, E. M., Winefordner, J. D., J. Agric. Food
  Chem., 27, 1233 (1979).
THANKS

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Understanding Luminescence Types and Techniques

  • 1. LUMINESENCE The term 'luminescence' was introduced in 1888 by Eilhard Wiedemann . “Luminescence is the emission of light by a substance. It occurs when an electron returns to the electronic ground state from an excited state and loses it's excess energy as a photon.” Luminescence spectroscopy is a collective name given to three related spectroscopic techniques. They are;  Molecular fluorescence spectroscopy  Molecular phosphorescence spectroscopy  Chemiluminescence spectroscopy
  • 2. TYPES OF LUMINESENCE  Bioluminescence  Chemiluminescence  Electrochemiluminescence  Crystalloluminescence  Electroluminescence  Mechanoluminescence  Triboluminescence  Fractoluminescence  Piezoluminescence  Radioluminescence  Sonoluminescence  Thermoluminescence
  • 3. PHOTOLUMINESENCE “Photoluminescence (PL) is the spontaneous emission of light from a material under optical excitation.” It is futher subdivided into two types a. Flourescence b. Phosphorescence
  • 4. ACTIVATION AND DEACTIVATION IN PHOSPHORESENCE  The absorption of a photon of suitable energy causes the molecule to get excited from the ground state to one of the excited states. This process is called as excitation or activation and is governed by Franck-Condon principle.  According to this principle, the electronic transition takes place so fast (~10-15 s) that the molecule does not get an opportunity to execute a vibration,  i.e., when the electrons are excited the internuclear distance does not change. • The basis for the principle is that the nuclei are very massive as compared to the electrons and therefore move very slowly.
  • 5. At the ground state , the molecular orbitals are occupied by two electrons. the spins of the two electrons in the same orbital must be antiparallel. This implies that the total spin, S, of the molecule in the ground state is zero [½ + ( ½)]. • This energy state is called “singlet state” and is labeled as S0. • The electron spins in the excited state achieved by absorption of radiation may either be parallel or antiparallel. Accordingly, this may be a triplet (parallel) or a singlet (antiparallel) state.
  • 6. The deactivation processes can be broadly categorized into two groups given below. • Nonradiative deactivation  Vibrational Relaxation  Internal Conversion  Intersystem Crossing • Radiative deactivation  Fluorescence  Phosphorescence
  • 8. DIFFERENCE BETWEEN PHOSPHORESCENCE AND FLUORESCENCE Phosphorescence Fluorescence  The emission could  The emission could proceed either from a proceed only from a singlet or triplet state. singlet state.  short-live electrons  longer lifetime of the (<10-5 s) in the excited excited state (second state of fluorescence to minutes)
  • 9. FLUORESCENCE AND PHOSPHORESCENCE  Fluorescence  Phosphorescence
  • 10. PHOSPHORESCENCE SPECTROSCOPY Phosphorescence Spectroscopy is the spectroscopic study of the radiation emitted by the lifetime of phosphorescence. Phosphorescence has been observed from a wide variety of compounds and is differentiated from fluorescence by the long-lived emission of light after extinction of the excitation source. The first analytical uses of phosphorescence were published in 1957 by Kiers et. al.
  • 11. FIG:SRAL2O4 ,PIGMENTS IN THE DARK AND THAN PIGMENTS IN THE DARK AFTER 4 MIN
  • 12. PHOSPHORIMETRY  Spectrophosphorimeter is similar to a Spectrofluorimeter except that the former instrument must be fitted with 1) a sample system which is maintained at liquid nitrogen temperature 2) A Rotating-shutter device commonly called a phosphoroscope and .
  • 13. SAMPLE PREPARATION  The majority of phosphorescence measurements are carried out in rigid media at the temperature of liquid nitrogen  The criteria for solvent selection are:  good solubility of the analyte  formation of a clear rigid glass at 77 K  low phosphorescence background (high purity)  For polar compounds, ethanol is an excellent solvent and small  For non-polar compounds, the most popular solvent is a mixture of diethyl ether, isopentane and ethanol in the ratio of 5:5:2 respectively  The samples are placed in a narrow quartz tube(internal diameter varying from 1 to 3 mm).  The dimensions are a compromise between too small a diameter and too large a diameter.  The sample tubes are placed in liquid nitrogen held in a quartz Dewar flask, and the latter placed in the sample holder known as a phosphoroscope.
  • 14. Phosphorescence can also be observed from solid samples at room temperature, and the compounds can be divided into two types.  The first includes inorganic salts and oxides such as the rare earths, europium and uranium  The second type of compounds are those which exhibit phosphorescence when absorbed onto certain substrates such as paper, cellulose, silica, etc.  Polar organic molecules, when absorbed onto filter paper from solutions containing 1 N NaOH and thoroughly dried, exhibit phosphorescence.  Studies have shown that the phosphorescence could be enhanced by the addition of heavy atoms, for example iodine, silver, lead
  • 16. INSTRUMENTATION  Excitation Source  Filters/Monochromators for excitation radiations  Phosphorscope(sample Cell)  Filters and Monochromators for emission  Detectors
  • 17. EXCITATION SOURCE  High intensity source of UV light are used  Lasers – A laser makes it possible to have narrow wavelength intervals that offer very high energy irradiation. This is useful when a large amount of energy is needed to produce the Phosphorescence in the sample.  Photodiodes – Photodiodes are specialized diodes that can be configured in a manner that allows electrons to flow towards the sample so that the excess energy excites the phosphorescent particles.  Xenon Arcs – Arcs of Xenon can produce the right amount of radiation for Phosphorescent materials.  Mercury Vapor – Since mercury vapor can create ultraviolet radiation when electrical current is passed through it, it is good for use with materials that shows Phosphorescence under the ultraviolet radiation. Care should be taken as Intense UV light is hazardous for health
  • 18.  Filters and monochromators used in a phosphorimeter device.  Filters  Absorption  Interfernce  Monochromators allow wavelength adjustment. Monochromators make it possible to do so with a diffraction grating.  The primary filters that excite the sample provide the appropriate wavelength  while the secondary filters monochromate the emitted light when sent to the detector.  Phosphoresence spectroscopy detectors may have a  single channel (single wavelength from sample)  or multiple channels (multiple wavelengths detection)
  • 19. PHOSPHOROSCOPE 1.The Becquerel or rotating disc phosphoroscope  A rotating disk excitation optical chopper, with three open and three larger opaque areas, is used to alternately excite the sample and allow phosphorescence to be measured.  By measuring the phosphorescence intensity at several time intervals along the emission decay curve, a recorder trace of the decay with respect to time can be produced.  The analytical precision and accuracy for quantitative measurements is improved by rotating the sample tube. This minimizes variation in the signal due to sample inhomogeniety resulting from imperfect glass formation at lowtemperatures .
  • 20. 2.The Rotating-Can Phosphoroscope:  It consists of hollow cylinder having one or more slit which are equally spaced in the circumference.  This is rotated by a variable-speed motor(>1000rpm)  when the rotating-can is rotated by a motor the sample is excited show fluorescence and phosphorescence  For Fluorescence The emission monochromator is blocked by the can so that fluorescence and scattered radiation cannot be detected.  As the can rotates, the excitation beam is blocked and the fluorescence and scattered radiation decay to a negligible amount.  Further rotation of the can will bring the window into alignment with the emission monochromator entrance slit and phosphorescence radiation will pass into the emission monochromator and onto the sample photomultiplier
  • 21.
  • 22. PULSED SOURCE-TIME RESOLVED PHOSPHORIMETRY  was first proposed by Fisher and Winefordner in 1972.  A pulsed source produces higher peak intensities than a continuously operated xenon lamp resulting in a greater peak phosphorescence emission intensity.  Pulsed source phosphorimetry has the advantage of time resolution compared with a mechanically modulated system permitting the analysis of organic phosphor with short lifetimes (0.1 to 50 microsec)  The xenon lamp produces a burst of energy with a width a half peak intensity of less than 10 μsec.  The signals from the sample photomultiplier are gated and both the  delay of the start of the gate after the start the flash  Timing is performed by a crystal clock and is highly accurate.  a quantum-corrected reference photomultiplier is used to monitor the flash intensity and the signals from th sample and reference
  • 23. FIG:SCHEMATIC DRAWING OF GATED PHOSPHORIMETER SETUP.
  • 24. THE PERKIN ELMER LS 55 LUMINESCENCE SPECTROMETER  It is a very versatile instrument that allows measurement of fluorescence, phosphorescence , chemiluminescence and bioluminescence of a liquid, solid, powder, or thin film sample  Fluorescence data are collected at the instant of the flash while phosphorescence data are collected in the dark period between each flash.
  • 25. APPLICATIONS OF PHOSPHORESCENCE SPECTROSCOPY  Pharmaceutical Applications  Clinical Applications  Environmental Applications  Forensic Applications  Entertainment Applications
  • 26. PHARMACEUTICAL APPLICATIONS  The majority of phosphorescence applications have been applied in the drug and pharmaceutical field and in the analysis of pesticides  A number of the sulphonamide class of drugs exhibit phosphorescence as do phenobarbital, cocaine, procaine, chlorpromazin and salicylic acid.
  • 27. CLINICAL APPLICATIONS  The phosphorescence intensity of the rare earths increases tremendously when they are covalently bound to certain molecules and this feature has been used in the analysis of transferin in blood  dual-wavelength phosphorimeter used to measure microvascular PO2 (µPO2) in different depths in tissue and demonstrates its use in rat kidney.
  • 28.
  • 29. Entertainment Applications  use of phosphor coated stamps and envelopes has appeared which gives a fascinating insight into the practical use of phosphorescence  The rare earths and uranyl elements phosphoresce and a number of them, particularly europium and terbium, are used as phosphors in lamps and TV tubes.
  • 30. ENVIRONMENTAL APPLICATIONS  Phosphorescence has been used in the detection of air and water-borne pollutants  for the analysis of impurities in polycyclic aromatic hydrocarbons and in petroleum products .
  • 31. CONCLUSION Although the applications of phosphorescence have been somewhat limited in the past, the introduction of new instrumentation and advances made in room temperature phosphorescence have lead to an increase in its use, particularly in clinical chemistry , the forensic, environmental and pharmaceutical fields.
  • 32. REFERENCES 1.Kiers, R.J., Britt, R.D., Wentworth, W.E., Anal. Chem., 29, 202 (1957). 2. Fluorescence Detection in Liquid Chromatography., Rhys Williams, A.T., PerkinElmer Limited (1980). 3. Schulman, E. M., Walling, C., J. Phys. Chem., 77, 902 (1973). 4. Hollifield, H. C., Winefordner, J. D., Anal. Chem., 40, 1759 (1968). 5. Zweidinger, R., Winefordner, J. D., Anal. Chem., 42, 639 (1970). 6. Fisher, R. P., Winefordner, J. D., Anal. Chem., 44, 948 (1972). 7. Harbaugh, K.F., O’Donnell, C. M., Winefordner, J. D., Anal. Chem., 45, 381 (1973.) 8. Sawicki, E., Pjaff, J. D., Anal. Chim. Acta., 32, 521 (1965). 9. Giffard, L. A., Miller, J. N., Burns, D. T., Bridges, J. W., J. Chromatog., 103, 15(1975). 10. de Lima, C. G., Nichola, E. M., Anal.Chem., 50, 1658 (1978). 11. O’Donnell, C. M., Winefordner, J. D., Clin. Chem., 21, 285 (1975).
  • 33. 12. Aaron, J. J., Winefordner, J. D., Anal.Chem., 44, 2127 (1972). 13. Vo. Dinh, T. Winefordner, J. D., Appl. Spec. Rev., 13, 261 (1977). 14. Saunders, L. B., Winefordner, J. D., Talanta, 16 407 (1969). 15. Aaron, J. J. Winefordner, J. D., Anal. Chem., 19, 21 (1972) 16. Hollifield, H. C., Winefordner, J. D., Talanta, 12, 860 (1965). 17. Winefordner, J. D., Latz, H. W., Anal. Chem., 35, 1517 (1963). 18. Perry, A. W., Winefordner, J. D., Anal. Chem., 43, 781 (1971). 19. Aaron, J. J., Kaleel, E. M., Winefordner, J. D., J. Agric. Food Chem., 27, 1233 (1979).