Refractometry of Living Cells

The principles underlying a new method of refractometry of living cells are discussed. The method was evolved from the chance observation that the amoebocytes of the blood of the earthworm, examined in their own blood, appeared bright instead of dark by positive phase-contrast microscopy. This was shown to be due to the presence of dissolved haemoglobin which raised the refractive index of the medium above that of the cytoplasm. In order to determine the refractive index of the latter it was only necessary to dilute the blood until the cytoplasm became virtually invisible. Non-pigmented proteins and other high molecular weight substances have now been substituted for haemoglobin. The nature of the initial observations suggested that if the cell could be regarded to a first approximation as being composed entirely of proteins, the cytoplasmic protein concentration could be equated to the protein concentration of the immersion medium which made the cell appear with minimum contrast. This would only be true if equal concentrations of different proteins in solution had the same refractive index. The nature of refractive index and its relationship to density are discussed and it is shown that for nearly all unconjugated proteins so far investigated the specific refraction increments (i.e. the increase in refractive index per 1 per cent, increase in concentration) have almost the same values (.00185±2 per cent.). The effects of many factors such as pH, salts, temperature, wavelength, concentration, and nature of the solvent are discussed. Since living cells contain substances other than proteins the specific refraction increments of protein derivatives, lipides, carbohydrates, and salts are considered and it is shown that the presence of moderate amounts of such substances is unlikely to affect the refractive index of cells to any great extent. It is suggested that the mean specific refraction increment of protoplasm should be taken as .0018 and that this value can be used in order to calculate the solid and water content of protoplasm from values of refractive index.

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Some problems concerning refractive index measurement by phase contrast microscopy using a PC coupled CCD camera

10.1117/12.519792 ◽

2003 ◽

Author(s):

Georgeta Sorohan ◽

Danut V. Ursu

Keyword(s):

Refractive Index ◽

Phase Contrast ◽

Ccd Camera ◽

Phase Contrast Microscopy ◽

Refractive Index Measurement ◽

Index Measurement ◽

Contrast Microscopy

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Direct measurement of the refractive index profile of phase gratings, recorded in silver halide holographic materials by phase-contrast microscopy

Applied Physics Letters ◽

10.1063/1.1629794 ◽

2003 ◽

Vol 83 (21) ◽

pp. 4282-4284 ◽

Cited By ~ 12

Author(s):

I. Bányász

Keyword(s):

Refractive Index ◽

Direct Measurement ◽

Phase Contrast ◽

Silver Halide ◽

Refractive Index Profile ◽

Phase Contrast Microscopy ◽

Index Profile ◽

Contrast Microscopy

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The Action of Formaldehyde on Living Cells as Studied by Phase-contrast Microscopy

Journal of Cell Science ◽

10.1242/jcs.s3-92.20.403 ◽

1951 ◽

Vol s3-92 (20) ◽

pp. 403-452

Author(s):

C. N.C. CRAWFORD ◽

R. BARER

Keyword(s):

Phase Contrast ◽

Morphological Changes ◽

Cytoplasmic Inclusion ◽

Living Cells ◽

Cell Swelling ◽

Phase Contrast Microscopy ◽

Chemical Action ◽

Short Period ◽

Contrast Microscopy ◽

Constant Observation

The morphological changes occurring when living cells are fixed in neutralized formaldehyde have been studied in detail with phase-contrast microscopy. The cells used were (i) salamander spermatogonia obtained from the teased testis, and (2) ssnail amoebocytes growing in tissue culture. The cells were mounted on a slide beneath a coverslip ringed with paraffin wax. Various strengths of formaldehyde made up in saline or distilled water were then introduced while the cells were kept under constant observation by phase-contrast microscopy. The morphological changes during the fixation process were observed for periods of at least 24 hours and the results recorded photographically. The main changes observed with aqueous formaldehyde were: A. Cell swelling or shrinkage. In general (e.g. with 5 per cent, formaldehyde) the cell tended to undergo (1) an initial short period of shrinkage, (2) a period of re-expansion followed by swelling, (3) a period of secondary shrinkage. The initial shrinkage appeared less in the amoebocytes than in the spermatogonia, but otherwise their volume changes were fairly similar. If the strength of formaldehyde was below 5 per cent, the initial shrinkage was very slight and subsequent swelling great. With 1 per cent, formaldehyde, sudden collapse of the cell followed swelling. With formalde-hyde concentrations above 10 per cent, the initial shrinkage was greater and was followed by little or no swelling. B. Formation of ‘bubbles’ from the cells. Clear bubble-like structures often emerged from the spermatogonia during fixation. They were most frequently formed in 5 per cent, formaldehyde. Increasing the strength of the formaldehyde decreased both the number and size of the ‘bubbles’. It is suggested that they may represent an escape of substance through a damaged cell boundary. Similar bubble-like swellings formed in the amoebocytes, but they usually seemed to remain within the cell processes. C. Nuclear changes. Changes in the size of the nucleus ran approximately parallel with those of the cell, but tended to be somewhat less and with different time relation-ships. With swelling the nucleoplasm became more homogeneous and with gross swelling the heterochromatic bodies disappeared. After prolonged fixation, when the nucleus may have undergone secondary shrinkage, pre-existing nuclear opacities became denser and new opacities sometimes appeared in previously homogeneous regions. Bubbles sometimes emerged from the nucleus. D. Changes in cytoplasmic structure. In general with prolonged fixation a fine granularity or reticular opacities formed in previously homogeneous cytoplasm. Clear vacuoles also appeared in the cytoplasm after fixation in the more concentrated solutions. The cytoplasmic inclusion bodies were usually well preserved and their appearance little altered. With formaldehyde made up in saline as opposed to water the initial shrinkage was increased and the subsequent swelling reduced. This effect was most pronounced with dilute formaldehyde. The addition of saline seemed to have little influence on changes in nuclear and cytoplasmic texture, and bubbling, though less in degree, still occurred. The significance of these observations is discussed in the light of modern views on the physico-chemical action of formaldehyde.

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The control of amplitude in phase-contrast microscopy

Proceedings of the Royal Society of London Series A - Mathematical and Physical Sciences ◽

10.1098/rspa.1947.0085 ◽

1947 ◽

Vol 190 (1022) ◽

pp. 422-426 ◽

Cited By ~ 12

Keyword(s):

Phase Contrast ◽

Living Cells ◽

Differential Staining ◽

Phase Contrast Microscopy ◽

Living Tissue ◽

The Past ◽

Contrast Microscopy ◽

Focus Image ◽

Dark Ground ◽

First Time

In the past the biologist has generally resorted to differential staining as a means of rendering visible slight non-homogeneities in his preparations. When such treatment was impracticable, as in the case of living cells, the alternatives were to study the out-of-focus image, to illuminate the specimen with very narrow' pencils (with a consequent loss of resolution), or to use dark-ground illumination. Phase contrast offers a means of converting slight changes of refractive index (with the consequent change of wave front) into corresponding changes of amplitude. The method possesses the advantages that the object is accurately focused, that the full aperture of the objective is used and that the eye is particularly sensitive to changes in amplitude. It also makes possible for the first time the detailed study at full aperture of transparent living tissue in place of the usual stained preparations which may have undergone considerable modification in the course of processing.

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