Literature DB >> 6166593

Errors in microdensitometry.

D J Goldstein.   

Abstract

Microdensitometric errors can originate in the instrument, in the specimen or in the human operator. Instrumental sources of systematic error mostly reduce the apparent integrated absorbance, especially of relatively small and highly absorbing objects. They can be assessed, minimized or eliminated by available techniques, but with modern apparatus are in general important only if results of high accuracy are required. Instrument errors include: (a) distributional error, due to the use of too large a measuring spot or the specimen being out of focus; (b) glare (stray light), due mainly to multiple reflections in the microscope objective; (c) monochromator error (the use of insufficiently pure light); (d) calibration errors; and (e) errors resulting from lack of photometric linearity, or the specimen absorbance exceeding the measuring range of the instrument. Specimen errors, including the problems of specificity and stoichiometry, are now the most important obstacles to a wider use of microdensitometry. The following selected topics are briefly discussed: fading; rate of staining; Beer's law deviations and the microdensitometry of opaque particles. Human errors include faulty logic, and failing to attempt an investigation because of anticipated difficulties which are in fact exaggerated or imaginary. The significance of microdensitometric results should, in general, be assessed by biological criteria rather than merely statistically; the use is urged of appropriate internal biological controls and standards wherever possible.

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Year:  1981        PMID: 6166593     DOI: 10.1007/BF01006883

Source DB:  PubMed          Journal:  Histochem J        ISSN: 0018-2214


  43 in total

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6.  Aspects of scanning microdensitometry. III. The monochromator system.

Authors:  D J Goldstein
Journal:  J Microsc       Date:  1975-09       Impact factor: 1.758

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Authors:  V James; D J Goldstein
Journal:  Br J Haematol       Date:  1974-09       Impact factor: 6.998

9.  Aspects of scanning microdensitometry. I. Stray light (glare).

Authors:  D J Goldstein
Journal:  J Microsc       Date:  1970       Impact factor: 1.758

10.  Nuclear DNA content of the emu.

Authors:  N G Martin
Journal:  Chromosoma       Date:  1974       Impact factor: 4.316

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  22 in total

1.  Quantitative determination of calcium-activated myosin adenosine triphosphatase activity in rat skeletal muscle fibres.

Authors:  C E Blanco; G C Sieck
Journal:  Histochem J       Date:  1992-07

Review 2.  The principle of determining relative enzyme activities by comparative kinetic microphotometry in situ.

Authors:  D Pette; H Reichmann
Journal:  Histochem J       Date:  1989 Sep-Oct

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Authors:  P Kugler; S Vogel; M Gehm
Journal:  Histochemistry       Date:  1988

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Review 5.  A user's guide for avoiding errors in absorbance image cytometry: a review with original experimental observations.

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Journal:  Histochem J       Date:  1994-01

Review 6.  Basic strategies for valid cytometry using image analysis.

Authors:  A Jonker; W J Geerts; P Chieco; A F Moorman; W H Lamers; C J Van Noorden
Journal:  Histochem J       Date:  1997-05

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Journal:  Histochem J       Date:  1986-07

8.  Reaction rate studies of glucose-6-phosphate dehydrogenase in rat tracheal epithelium; the effect of section thickness.

Authors:  R G Butcher
Journal:  Histochemistry       Date:  1984

9.  Reaction rate studies of glucose-6-phosphate dehydrogenase activity in sections of rat liver using four tetrazolium salts.

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Journal:  Histochem J       Date:  1985-09

10.  Cytophotometry of glucose-6-phosphate dehydrogenase activity in individual cells.

Authors:  C J Van Noorden; J Tas; I M Vogels
Journal:  Histochem J       Date:  1983-06
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