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1.
《Biotechnic & histochemistry》2013,88(1):07-20
1. An attempt has been made to apply Loeb's concept of the amphoteric nature of proteins for the discrimination of suspected hemoglobiniferous substances from known hemoglobiniferous substances according to their reactions to acid and basic dyes with reference to the isoelectric point of hemoglobin (pH 6.8).2. The substances in the cytoplasm of known hemoglobiniferous cells (red blood corpuscles, normoblasts and erythroblasts) of the lymph nodes, spleen and bone marrow of the albino rat, when suspended in buffered dye-sucrose solutions, retain eosin on the acid side of pH 7.0, but the substances of the Russell bodies, suspected of being hemoglobiniferous, do not retain eosin at all; and the cytoplasm of the plasma cells, also alleged to be slightly hemoglobiniferous, only retains eosin on the acid side of pH 6.4.3. The only basic dye used which did not precipitate in buffer solutions was methylene blue. This did not react with hemoglobin in accordance with Loeb's concept, because it did not penetrate mature red blood corpuscles and in those immature erythrocytes which it did penetrate it was precipitated by the reticulum.4. Therefore, from the results obtained with the acid dye, it is tentatively concluded that the substance in the Russell bodies and in the cytoplasm of the plasma cells are not hemoglobiniferous because they do not react as do the substances in known hemoglobiniferous cells with reference to the isoelectric point of hemoglobin.5. More investigation, however, must be carried out on both fresh and fixed material before a final unequivocal answer can be made to this problem. 相似文献
2.
H. A. Davenport 《Biotechnic & histochemistry》1934,9(2):49-52
The fixing action of 10% formalin solution alone and with formic, acetic, propionic, butyric, lactic, monochloracetic, dichloracetic, or trichloracetic acid was studied by means of stains with silver, osmic acid and cresyl violet. The following conclusions were reached:
1. In general, better fixation and staining was obtained with acid than without.
2. Less difference was seen in comparing one acid with another than was expected before the experiments were made.
3. Propionic, butyric, and dichloracetic showed no promise of having practical value.
4. Formic and monochloracetic acids as modifiers gave superior stains with osmic acid, while silver and cresyl violet stains of the same material were about equal to those made from formalin-acetic fixed material.
5. Lactic acid caused somewhat more distortion of tissue elements than the others but was compatible with good staining.
6. Acetic acid was most effective in concentrations of 3 to 5% while the stronger acids such as formic, monochloracetic, lactic and trichloracetic were effective in concentrations of 0.5 to 1%. 相似文献
1. In general, better fixation and staining was obtained with acid than without.
2. Less difference was seen in comparing one acid with another than was expected before the experiments were made.
3. Propionic, butyric, and dichloracetic showed no promise of having practical value.
4. Formic and monochloracetic acids as modifiers gave superior stains with osmic acid, while silver and cresyl violet stains of the same material were about equal to those made from formalin-acetic fixed material.
5. Lactic acid caused somewhat more distortion of tissue elements than the others but was compatible with good staining.
6. Acetic acid was most effective in concentrations of 3 to 5% while the stronger acids such as formic, monochloracetic, lactic and trichloracetic were effective in concentrations of 0.5 to 1%. 相似文献
3.
David L. Sargent 《Biotechnic & histochemistry》1936,11(2):49-52
A modification of Donaldson's iodine-eosin stain for staining intestinal protozoa is presented. This modification consists of using high dilutions of colloidal iodine (Chandler)2 instead of Lugol's solution as well as high dilutions of eosin. A better resolution of the external and internal structures is brought about by the new method.
The procedure is as follows: A portion of the fecal material to be examined is suspended in a 0.6% salt solution; the suspension should be of a consistency so that one drop will make a satisfactory microscope mount under a cover glass. To ten parts of this suspension, in a test tube, is added one part of the stain which is prepared as follows:—
10 parts of distilled water
6 parts of a suspension of colloidal iodine (Chandler) containing 4% iodine—20% iodine suspensoid, Merck
1 part of a 10% water solution of anilin red, Merck (eosin yellowish)
Technicians will find, because iodine in the form of colloidal iodine is readily released to the organisms, that the use of this material is far superior to Lugol's solution hi carrying out the technic for staining intestinal protozoa in the study of fresh mount preparations. Not only are organisms more deeply stained with iodine but by eosin as well, even when employed in high dilutions. 相似文献
The procedure is as follows: A portion of the fecal material to be examined is suspended in a 0.6% salt solution; the suspension should be of a consistency so that one drop will make a satisfactory microscope mount under a cover glass. To ten parts of this suspension, in a test tube, is added one part of the stain which is prepared as follows:—
10 parts of distilled water
6 parts of a suspension of colloidal iodine (Chandler) containing 4% iodine—20% iodine suspensoid, Merck
1 part of a 10% water solution of anilin red, Merck (eosin yellowish)
Technicians will find, because iodine in the form of colloidal iodine is readily released to the organisms, that the use of this material is far superior to Lugol's solution hi carrying out the technic for staining intestinal protozoa in the study of fresh mount preparations. Not only are organisms more deeply stained with iodine but by eosin as well, even when employed in high dilutions. 相似文献
4.
Spinal cord of cat and rabbit was stained, after experimental lesions, by variations of Marchi's method. The following conclusions were drawn:
1. The presence of an oxidizing agent (K2Cr2O7, NaIO3, or KCIO3) in the osmic acid solution is of primary importance and a preliminary oxidation in Mueller's fluid is unnecessary or even detrimental.
2. Acetic acid added to Marchi's fluid, accentuates the action of the oxidizing agent in restraining the staining of normal myelin.
3. Too high concentration of oxidizing agent or of acid may inhibit staining of degenerating myelin.
4. Marchi's and Busch's methods have been modified as follows: Fix one day in 10% formalin and transfer without washing to the staining mixture, either A or B. Staining mixture A: Marchi's fluid plus 1 to 3% glacial acetic acid. B: An aqueous solution containing KCIO3 0.25%, osmic acid 0.33%, and acetic acid 1%. Stain about one week. These methods worked on spinal cord and medulla, but cannot be recommended for brain.
5. The detrimental effects of long post mortem autolysis or of prolonged fixation in formalin may be counteracted to some degree by increasing the concentration of the acid in Marchi's fluid up to 5% or of the KCIO3 up to 0.4% in the modified Busch's fluid. 相似文献
1. The presence of an oxidizing agent (K2Cr2O7, NaIO3, or KCIO3) in the osmic acid solution is of primary importance and a preliminary oxidation in Mueller's fluid is unnecessary or even detrimental.
2. Acetic acid added to Marchi's fluid, accentuates the action of the oxidizing agent in restraining the staining of normal myelin.
3. Too high concentration of oxidizing agent or of acid may inhibit staining of degenerating myelin.
4. Marchi's and Busch's methods have been modified as follows: Fix one day in 10% formalin and transfer without washing to the staining mixture, either A or B. Staining mixture A: Marchi's fluid plus 1 to 3% glacial acetic acid. B: An aqueous solution containing KCIO3 0.25%, osmic acid 0.33%, and acetic acid 1%. Stain about one week. These methods worked on spinal cord and medulla, but cannot be recommended for brain.
5. The detrimental effects of long post mortem autolysis or of prolonged fixation in formalin may be counteracted to some degree by increasing the concentration of the acid in Marchi's fluid up to 5% or of the KCIO3 up to 0.4% in the modified Busch's fluid. 相似文献
5.
Elbert C. Cole 《Biotechnic & histochemistry》1936,11(2):45-47
1. Tissues stained intra vitam with methylene blue are fixed in a 10% ammonium molybdate solution in physiological saline (or sea water if the tissue is from a marine animal). Fixation time is kept to a minimum. Washing also is reduced to a minimum.
2. Excess fluids are removed from tissues by blotting with a paper or cloth towel before they are put into the succeeding solution. Tissues are taken from the wash water, blotted and placed in a mixture of equal parts of absolute ethyl alcohol and n-butyl alcohol for 30 minutes. They are then blotted and transferred to n-butyl alcohol for 30 minutes. After blotting they are placed in a mixture of one part methyl salicylate and four parts xylene until cleared. Tissues may be mounted whole or prepared for sectioning by embedding in paraffin in the usual way.
3. Tissues fixed, washed, dehydrated and cleared as described retain nearly all of the stain; the time required is greatly reduced; there is no need to chill the dehydrating solutions; cell distortion is much reduced. 相似文献
2. Excess fluids are removed from tissues by blotting with a paper or cloth towel before they are put into the succeeding solution. Tissues are taken from the wash water, blotted and placed in a mixture of equal parts of absolute ethyl alcohol and n-butyl alcohol for 30 minutes. They are then blotted and transferred to n-butyl alcohol for 30 minutes. After blotting they are placed in a mixture of one part methyl salicylate and four parts xylene until cleared. Tissues may be mounted whole or prepared for sectioning by embedding in paraffin in the usual way.
3. Tissues fixed, washed, dehydrated and cleared as described retain nearly all of the stain; the time required is greatly reduced; there is no need to chill the dehydrating solutions; cell distortion is much reduced. 相似文献
6.
Alexander V. Tolstoouhov 《Biotechnic & histochemistry》1928,3(2):49-56
As was reported in a previous paper,1 staining properties depend on the chemical composition of the tissues and on the strength of the dyes themselves. Applying mixtures of basic and acid dye on tissues (methylene blue, eosin Y) at different pH-values, it is possible to find differences in the isoelectric points of the nuclei and cytoplasm of different tissues. For example, the nucleus of polymorphonuclear cells of the blood consists of the most acid protein, with an isoelectric point around pH 2.5, while the nucleus of lymphatic tissues has an isoelectric point of about pH 4.0, and that of connective tissue about pH 3.4.
With a knowledge of the above, a constant method of staining at various pH-values was used to study the effect of different fixing fluids on the staining properties of the tissues. In this way it was found that many fixing fluids gave very stable compounds with tissue proteins, and that they almost permanently change the chemical composition (i.e. the staining properties of the tissues). In some instances, these changes can be easily explained from the regular chemical standpoint. For example, formalin forms inert compounds with amino groups of the amino acids of proteins and in this way it makes the tissue proteins more acid, i.e. it moves the isoelectric point of the proteins toward a lower pH-value. The same is true in the case of the polivalent acids. The bivalent heavy metals such as mercury, on the contrary, it is assumed, combine with carboxyi groups of amino acids and in this way move the isoelectric point of the proteins toward a higher pH. 相似文献
With a knowledge of the above, a constant method of staining at various pH-values was used to study the effect of different fixing fluids on the staining properties of the tissues. In this way it was found that many fixing fluids gave very stable compounds with tissue proteins, and that they almost permanently change the chemical composition (i.e. the staining properties of the tissues). In some instances, these changes can be easily explained from the regular chemical standpoint. For example, formalin forms inert compounds with amino groups of the amino acids of proteins and in this way it makes the tissue proteins more acid, i.e. it moves the isoelectric point of the proteins toward a lower pH-value. The same is true in the case of the polivalent acids. The bivalent heavy metals such as mercury, on the contrary, it is assumed, combine with carboxyi groups of amino acids and in this way move the isoelectric point of the proteins toward a higher pH. 相似文献
7.
Root tips of Liriodendron Tulipifera forming with a fungus of the Mycelium Radicis group an endotrophic mycorrhiza, were subjected to several different fixations in which the action of cationic chromium and anionic chromium were compared. Anionic chromium in the form of chromic acid was combined with several substituted benzene compounds while cationic chromium in the form of chromic sulfate (Cr2(SO4)3·15 H2O) in 4% formaldehyde (HCHO) was used with the same ring compounds. In addition, several fixatives not containing chromium were tested.
Five percent chromic sulfate (Cr2(SO4)2·15 H2O) in 4% formaldehyde (HCHO) or in 1% osmic acid with saturated aqueous salicylic and/or picric acid preserved the histological and cytological details of the mycorrhiza, as was clearly demonstrated when followed by staining in 3% acetic acid saturated with orseillin BB and counterstained with 1% crystal violet in clove oil.
Two percent ferric chloride (Fe Cl3) in 4% formaldehyde showed the relationship of the tannin contents of the cells to the invading hyphae when followed by suitable staining.
Cationic chromium appeared to be superior to anionic chromium in preserving cell walls as well as the general histologic features of the material investigated. 相似文献
Five percent chromic sulfate (Cr2(SO4)2·15 H2O) in 4% formaldehyde (HCHO) or in 1% osmic acid with saturated aqueous salicylic and/or picric acid preserved the histological and cytological details of the mycorrhiza, as was clearly demonstrated when followed by staining in 3% acetic acid saturated with orseillin BB and counterstained with 1% crystal violet in clove oil.
Two percent ferric chloride (Fe Cl3) in 4% formaldehyde showed the relationship of the tannin contents of the cells to the invading hyphae when followed by suitable staining.
Cationic chromium appeared to be superior to anionic chromium in preserving cell walls as well as the general histologic features of the material investigated. 相似文献
8.
W. N. Steil 《Biotechnic & histochemistry》1936,11(3):99-100
After the blood smear is treated for the proper length of time with Wright's stain, neutral distilled water is used for diluting the stain. After the slide has been treated with neutral distilled water until the smear becomes pinkish it is then treated with pure absolute methyl alcohol which destains the plasma. Neutral distilled water is again kept on the mount until the corpuscles are well stained. Then the slide is dehydrated with absolute ethyl alcohol, cleared with clove oil and completed in the usual way.
Blood smears of different groups of vertebrates were uniformly brilliantly stained with the above technic.
Several lots of Wright's dry stain have been tested with the modified technic and no difficulties have been encountered in its application. 相似文献
Blood smears of different groups of vertebrates were uniformly brilliantly stained with the above technic.
Several lots of Wright's dry stain have been tested with the modified technic and no difficulties have been encountered in its application. 相似文献
9.
Following experimental lesions, spinal cords of cats and rabbits were fixed with acid, neutral, and alkaline solutions. Staining was limited to a chromate-osmic (Marchi's) solution and a chlorate-osmic solution. The following conclusions were drawn:
The presence of an acid in the fixative caused normal myelin sheaths to stain. This effect was reduced by washing tissues before staining, by adding acetic acid to the stain, or by employing a non-formalin fixative. It was, however, at no time entirely obviated.
A study was made of the granular deposits which occur in nearly all Marchi preparations and which are especially confusing if very light backgrounds are obtained.
The staining reactions of the granular deposits were very similar to those of degenerating myelin but some suppression of the granules was obtained by adding KCIO3 to the formalin fixative. 相似文献
The presence of an acid in the fixative caused normal myelin sheaths to stain. This effect was reduced by washing tissues before staining, by adding acetic acid to the stain, or by employing a non-formalin fixative. It was, however, at no time entirely obviated.
A study was made of the granular deposits which occur in nearly all Marchi preparations and which are especially confusing if very light backgrounds are obtained.
The staining reactions of the granular deposits were very similar to those of degenerating myelin but some suppression of the granules was obtained by adding KCIO3 to the formalin fixative. 相似文献
10.
11.
《Biotechnic & histochemistry》1945,20(1):27-32
LEGGETT, W. F. Ancient and Medieval Dyes. 5 × 8 in. 96 pp. Cloth. Chemical Publishing Co., Brooklyn, N. Y. 1944. $2.25.
Microtechnic In General. McCARTNEY, J. E. A new immersion oil “polyric”. J. Path. & Bact., 56, 265-6. 1944.
NICKERSON, MARK. A dry ice freezing unit for rotary microtomes. Science, 100, 177-8. 1944.
Dyes And Thedx Biological Uses. BERGEIM, FRANK H., and BRAKER, WILLIAM. Homosulfanilamides. J. Amer. Chem. Soc., 66, 1459. 1944.
CALDWELL, W. T., TYSON, F. T., and LAUER, LOTHAR. Substituted 2-sulfonamido-5-aminopyridines. II. J. Amer. Chem. Soc., 66, 1479. 1944.
JOHNS, C. K. Dye concentration in resazurin tablets. Amer. J. Pub. Health, 34, 955-8. 1944.
SMITH, WINSLOW WHITNEY. Relative sensitivity of different phases of growth curve of Bact. salmonicida to alkaline acriflavine. Proc. Soc. Exp. Biol. & Med., 56, 240-2. 1844.
VAN ARENDONK, A. M., and SHOULE, H. A. Dialkylaminoalkyl derivatives of substituted quinolines and quinaldines. J. Amer. Chem. Soc., 66, 1284. 1944.
WHEELER, KEITH, and DEGERING, E. F. Preparation and properties of certain derivatives of sulfamide. J. Amer. Chem. Soc., 66, 1242. 1944.
Animal Microtechnic. BOARDMAN, EDWARD T. Methods for collecting ticks for study and delineation. J. Parasitology, 30, 57-9. 1944.
DICKIE, MARGARET M. A new differential stain for mouse pituitary. Science, 100, 297-8. 1944.
GOVAN, A. D. TELFORD. Fat staining by Sudan dyes suspended in watery media. J. Path. & Bact., 56, 262-4. 1944.
LILLIE, R. D., and ASHBURN, L. L. Supersaturated solutions of fat stains in dilute isopropanol for demonstration of acute fatty degenerations not shown by Herxheimer technic. Arch. Path., 36, 432. 1943.
MULLEN, J. P. A convenient and rapid method for staining glycogen in paraffin sections with Best's carmine stain. Amer. J. Clin. Path., Tech. Sect., 8, 9-10. 1944.
NYKA, W. A method for staining the rickettsiae of typhns in histological sections. J. Path. & Bact., 56, 264. 1944.
POPPER, HANS, GYORGY, PAUL, and GOLDBLATT, H. Fluorescent material (ceroid) in experimental nutritional cirrhosis. Arch. Path., 37, 161. 1944.
SMALL, C. S., and SCHULTZ, M. A. Sustaining faded tissue sections. Amer. J. Clin. Path., Tech. Sect., 7, 66-7. 1943.
YOFFEY, J. M., and PARNELL, J. The lymphocyte content of rabbit bone marrow. J. Anat., 78, 109-12. 1944.
ZIEGLER, E. E. Hematoxylin-eosin tissue stain. An improved, rapid, and uniform technic. Arch. Path., 37, 68. 1044.
Plant Microtechnic. HAASIS, FERDINAND W. Staining rubber in ground or milled plant tissues. Ind. and Eng. Chem., Anal. Ed., 16, 480. 1944.
PARRIS, G. K. A simple nuclear stain and staining technique for Helminthosporia. Phytopathology, 34, 700. 1944.
Microorganisms. DARZINS, E. Rickettsienstudien. Zentbl. Bakl., Abt. I, Orig., 151, 18-20. 1943.
GOHAR, M. A. A staining method for Corynebacterium diphtheriae. J. Bact., 47, 575. 1944.
GRAY, P. H. H. Two-stain method for direct bacteria count. J. Milk Techn., 6, 76. 1943. 相似文献
Microtechnic In General. McCARTNEY, J. E. A new immersion oil “polyric”. J. Path. & Bact., 56, 265-6. 1944.
NICKERSON, MARK. A dry ice freezing unit for rotary microtomes. Science, 100, 177-8. 1944.
Dyes And Thedx Biological Uses. BERGEIM, FRANK H., and BRAKER, WILLIAM. Homosulfanilamides. J. Amer. Chem. Soc., 66, 1459. 1944.
CALDWELL, W. T., TYSON, F. T., and LAUER, LOTHAR. Substituted 2-sulfonamido-5-aminopyridines. II. J. Amer. Chem. Soc., 66, 1479. 1944.
JOHNS, C. K. Dye concentration in resazurin tablets. Amer. J. Pub. Health, 34, 955-8. 1944.
SMITH, WINSLOW WHITNEY. Relative sensitivity of different phases of growth curve of Bact. salmonicida to alkaline acriflavine. Proc. Soc. Exp. Biol. & Med., 56, 240-2. 1844.
VAN ARENDONK, A. M., and SHOULE, H. A. Dialkylaminoalkyl derivatives of substituted quinolines and quinaldines. J. Amer. Chem. Soc., 66, 1284. 1944.
WHEELER, KEITH, and DEGERING, E. F. Preparation and properties of certain derivatives of sulfamide. J. Amer. Chem. Soc., 66, 1242. 1944.
Animal Microtechnic. BOARDMAN, EDWARD T. Methods for collecting ticks for study and delineation. J. Parasitology, 30, 57-9. 1944.
DICKIE, MARGARET M. A new differential stain for mouse pituitary. Science, 100, 297-8. 1944.
GOVAN, A. D. TELFORD. Fat staining by Sudan dyes suspended in watery media. J. Path. & Bact., 56, 262-4. 1944.
LILLIE, R. D., and ASHBURN, L. L. Supersaturated solutions of fat stains in dilute isopropanol for demonstration of acute fatty degenerations not shown by Herxheimer technic. Arch. Path., 36, 432. 1943.
MULLEN, J. P. A convenient and rapid method for staining glycogen in paraffin sections with Best's carmine stain. Amer. J. Clin. Path., Tech. Sect., 8, 9-10. 1944.
NYKA, W. A method for staining the rickettsiae of typhns in histological sections. J. Path. & Bact., 56, 264. 1944.
POPPER, HANS, GYORGY, PAUL, and GOLDBLATT, H. Fluorescent material (ceroid) in experimental nutritional cirrhosis. Arch. Path., 37, 161. 1944.
SMALL, C. S., and SCHULTZ, M. A. Sustaining faded tissue sections. Amer. J. Clin. Path., Tech. Sect., 7, 66-7. 1943.
YOFFEY, J. M., and PARNELL, J. The lymphocyte content of rabbit bone marrow. J. Anat., 78, 109-12. 1944.
ZIEGLER, E. E. Hematoxylin-eosin tissue stain. An improved, rapid, and uniform technic. Arch. Path., 37, 68. 1044.
Plant Microtechnic. HAASIS, FERDINAND W. Staining rubber in ground or milled plant tissues. Ind. and Eng. Chem., Anal. Ed., 16, 480. 1944.
PARRIS, G. K. A simple nuclear stain and staining technique for Helminthosporia. Phytopathology, 34, 700. 1944.
Microorganisms. DARZINS, E. Rickettsienstudien. Zentbl. Bakl., Abt. I, Orig., 151, 18-20. 1943.
GOHAR, M. A. A staining method for Corynebacterium diphtheriae. J. Bact., 47, 575. 1944.
GRAY, P. H. H. Two-stain method for direct bacteria count. J. Milk Techn., 6, 76. 1943. 相似文献
12.
James Boyles Rogers 《Biotechnic & histochemistry》1935,10(4):135-138
An arrangement of apparatus for applying micro-manipulative procedures to cells in living mammals is described. It was found satisfactory for manipulation of pericapillary cells and capillary endothelium in the greater omentum of the cat.
An animal board, a Bausch and Lomb triple purpose micro-projector and a double Fitz micro-manipulator were mounted on a spring platform. The micro-needles were drawn from Pyrex rods by hand. The stage of the microscope was modified to protect the condenser from fluids. Warm saline solution was carried to the exposed omentum thru flexible rubber tubing.
The use of a micro-dissection chamber which immobilized the part of the omentum under manipulation is explained. The construction of this chamber is shown by diagrams. A camera support was bolted to the base of the micro-manipulator.
The arrangement of apparatus is shown by a photograph. 相似文献
An animal board, a Bausch and Lomb triple purpose micro-projector and a double Fitz micro-manipulator were mounted on a spring platform. The micro-needles were drawn from Pyrex rods by hand. The stage of the microscope was modified to protect the condenser from fluids. Warm saline solution was carried to the exposed omentum thru flexible rubber tubing.
The use of a micro-dissection chamber which immobilized the part of the omentum under manipulation is explained. The construction of this chamber is shown by diagrams. A camera support was bolted to the base of the micro-manipulator.
The arrangement of apparatus is shown by a photograph. 相似文献
13.
Procedures having enhanced reliability over older methods for both Bielschowsky and Cajal types of stain are described.
Fixation of embryos in a solution containing 4% formaldehyde and 0.5% trichloracetic acid greatly improved the staining of neural elements by Bielschowsky's method.
Among the variations of Cajal's type of staining tried, a modification of Ranson's pyridin-silver method gave the most complete staining of neurofibrillar elements. Washing for 0.5 to 1 hour after silver impregnation and shortening of the reduction time from 24 to 4 hours corrected the tendency of the method to overstain. 相似文献
Fixation of embryos in a solution containing 4% formaldehyde and 0.5% trichloracetic acid greatly improved the staining of neural elements by Bielschowsky's method.
Among the variations of Cajal's type of staining tried, a modification of Ranson's pyridin-silver method gave the most complete staining of neurofibrillar elements. Washing for 0.5 to 1 hour after silver impregnation and shortening of the reduction time from 24 to 4 hours corrected the tendency of the method to overstain. 相似文献
14.
《Free radical research》1998,28(3):353-356
Oxygen, Gene expression and Cellular Function, Vol 105 Lung Biology in Health and Disease L. B. Clerch and D. J. Massaro Marcel Dekker, 1997
Food and Free Radicals Edited by Midori Hiramatsu, Toshikazu Yoshikawa and Masayosu Inoue Plenum Press, 1997, ISBN 0-306-45493-9 vii + 169 pages
Preventing Coronary Heart Disease: The Role of Antioxidants, Vegetables and Fruit Ed Lesley Rogers and Imogen Sharp National Heart Forum 1997 The Stationery Office London
Inducible Gene Expression Volume 1 Environmental Stresses and Nutrients Volume 2 Hormonal Signals Ed by PA Baeuerle, Birkhauser Verlag AG, Basel, 1997
Antioxidants in Science, Technology, Medicine and Nutrition Gerald Scott Albion Chemical Science Series, Ellis Horwoood Publishing Ltd, Chichester, UK, 1997
Flavonoids in Health and Diseases Eds C A Rce-Evans and L Packer Marcel Dekker Inc, New York, 1997 相似文献
Food and Free Radicals Edited by Midori Hiramatsu, Toshikazu Yoshikawa and Masayosu Inoue Plenum Press, 1997, ISBN 0-306-45493-9 vii + 169 pages
Preventing Coronary Heart Disease: The Role of Antioxidants, Vegetables and Fruit Ed Lesley Rogers and Imogen Sharp National Heart Forum 1997 The Stationery Office London
Inducible Gene Expression Volume 1 Environmental Stresses and Nutrients Volume 2 Hormonal Signals Ed by PA Baeuerle, Birkhauser Verlag AG, Basel, 1997
Antioxidants in Science, Technology, Medicine and Nutrition Gerald Scott Albion Chemical Science Series, Ellis Horwoood Publishing Ltd, Chichester, UK, 1997
Flavonoids in Health and Diseases Eds C A Rce-Evans and L Packer Marcel Dekker Inc, New York, 1997 相似文献
15.
《Biotechnic & histochemistry》1949,24(3):193-194
Officers
President, H. J. Conn, Box 269, Geneva, N. Y. (representing Society of American Bacteriologists.)
Vice-President, W. F. Windle, University of Pennsylvania, Philadelphia, Pa. Secretary, S. I. Kornhauser, University of Louisville Medical School, Louisville
Ky. Treasurer, E. H. Stotz, University of Rochester, School of Medicine, Rochester
N. Y. (representing American Chemical Society.) 相似文献
President, H. J. Conn, Box 269, Geneva, N. Y. (representing Society of American Bacteriologists.)
Vice-President, W. F. Windle, University of Pennsylvania, Philadelphia, Pa. Secretary, S. I. Kornhauser, University of Louisville Medical School, Louisville
Ky. Treasurer, E. H. Stotz, University of Rochester, School of Medicine, Rochester
N. Y. (representing American Chemical Society.) 相似文献
16.
Among methods used for a study of nuclear details in the development of pollen grains, the following were found to be very satisfactory: (1) warming the entire grains in aceto-carmine and then clearing with chloral hydrate; (2) making smear preparations stained with crystal-violet-iodine or iron alum hematoxylin. For paraffin sections, a counterstain with dilute alcoholic erythrosin is often very useful after the usual iron hematoxylin technic.
A method of making cultures of pollen tubes on slides coated with thin films of sugar agar is described in detail. The tubes can be fixed by immersing the slide in formol-acetic-alcohol and then stained by any desired schedule. Iron alum hematoxylin was found to be the most satisfactory, but the Feulgen reaction is very valuable in such cases where the nuclei are obscured by the density of the pollen tube cytoplasm. Living pollen tubes can be kept under observation by dissolving a small quantity of neutral red or other vital stain in the sugar agar before it is spread on the slide.
For studying stages in fertilization or gametogenesis, styles should be fixed and sectioned only after a preliminary study with iodine-chloral-hydrate or safranin-anilin-blue or aceto-carmine. Once the extent to which pollen tubes grow in a given time in the stylar tissues has been determined, it is possible to fix material with some knowledge of what it is going to show.
Some other methods, that have not been tried by the authors but appear to be valuable, are also briefly described. 相似文献
A method of making cultures of pollen tubes on slides coated with thin films of sugar agar is described in detail. The tubes can be fixed by immersing the slide in formol-acetic-alcohol and then stained by any desired schedule. Iron alum hematoxylin was found to be the most satisfactory, but the Feulgen reaction is very valuable in such cases where the nuclei are obscured by the density of the pollen tube cytoplasm. Living pollen tubes can be kept under observation by dissolving a small quantity of neutral red or other vital stain in the sugar agar before it is spread on the slide.
For studying stages in fertilization or gametogenesis, styles should be fixed and sectioned only after a preliminary study with iodine-chloral-hydrate or safranin-anilin-blue or aceto-carmine. Once the extent to which pollen tubes grow in a given time in the stylar tissues has been determined, it is possible to fix material with some knowledge of what it is going to show.
Some other methods, that have not been tried by the authors but appear to be valuable, are also briefly described. 相似文献
17.
Henry C. Waterman 《Biotechnic & histochemistry》1934,9(1):23-31
In Note I are pointed out certain chemical difficulties which stand in the way of experiments on chromium fixation in alcoholic media; also a procedure is described by means of which these difficulties may be avoided in the preparation of a chrome-alcohol stock solution.
In Note II it is suggested that the properties of OsO4 most important in the quick-killing effect conferred by this adjuvant upon aqueous chromic reagents are probably, in addition to its high toxicity, its volatility and its oxidant action. Volatile, toxic oxidants which do not attack alcohol are therefore discussed briefly, with reference especially to their use as quick-killing adjuvants in chrome-alcohol reagents. Iodine is noted as probably the most important inorganic possibility. Reasons are stated for considering the quinones the most promising of numerous possible organic compounds.
Results of fixations of Vicia faba root tips in nine variations of the proportions of acetic acid and iodine in a chrome-alcohol-aceticiodine combination are described. The chrome-alcohol-iodine reagents which proved best proportioned for V. faba root tips preserved some details of the chromosomes better than does Bouin's solution, but did not make certain details of the early prophase as clear as does Benda's modification of the Flemming reagent, according to a comparison with Sharp's figures of Bouin and Benda preparations of root tips of the same species. 相似文献
In Note II it is suggested that the properties of OsO4 most important in the quick-killing effect conferred by this adjuvant upon aqueous chromic reagents are probably, in addition to its high toxicity, its volatility and its oxidant action. Volatile, toxic oxidants which do not attack alcohol are therefore discussed briefly, with reference especially to their use as quick-killing adjuvants in chrome-alcohol reagents. Iodine is noted as probably the most important inorganic possibility. Reasons are stated for considering the quinones the most promising of numerous possible organic compounds.
Results of fixations of Vicia faba root tips in nine variations of the proportions of acetic acid and iodine in a chrome-alcohol-aceticiodine combination are described. The chrome-alcohol-iodine reagents which proved best proportioned for V. faba root tips preserved some details of the chromosomes better than does Bouin's solution, but did not make certain details of the early prophase as clear as does Benda's modification of the Flemming reagent, according to a comparison with Sharp's figures of Bouin and Benda preparations of root tips of the same species. 相似文献
18.
《Free radical research》1996,25(5):455-459
The Biology of Nitric Oxide, vol. 3. Physiological and Clinical Aspects; vol. 4. Enzymology, Biochemistry and Immunology, Portland Press, 1994
Mitochondrial Diseases Editors: L. Ernster, R. Luft and S. Orrenius Publishers: Elsevier
Biothiols in Health and Disease Editors: Lester Packer & Enrique Cadenas Publishers: Marcel Dekker, Inc. 相似文献
Mitochondrial Diseases Editors: L. Ernster, R. Luft and S. Orrenius Publishers: Elsevier
Biothiols in Health and Disease Editors: Lester Packer & Enrique Cadenas Publishers: Marcel Dekker, Inc. 相似文献
19.
J. A. De Tomasi Abstract Editor 《Biotechnic & histochemistry》1938,13(4):169-173
Microscope and Other Apparatus: Bernard, J. E. The principles of fluorescence microscopy. J. Royal Micro. Soc., 57, 256-9. 1937.
Wrighton, H. A new light source for microscopy. J. Royal Micro. Soc., 57, 260-1. 1938.
Microtechhic in general: Comandon, J. and De Fonbrune, P. La chambre $aG huile. Ses avantages pour l'$eGtude des microorganisms vivants, la culture des tissus et la micromanipulation. Ann. Inst. Pasteur, 60, 113-41. 1938. 相似文献
Wrighton, H. A new light source for microscopy. J. Royal Micro. Soc., 57, 260-1. 1938.
Microtechhic in general: Comandon, J. and De Fonbrune, P. La chambre $aG huile. Ses avantages pour l'$eGtude des microorganisms vivants, la culture des tissus et la micromanipulation. Ann. Inst. Pasteur, 60, 113-41. 1938. 相似文献
20.
A method is described for preparing cake crumb for sectioning and staining. Previous to embedding, the fat was stained and fixed by exposing small blocks of cake to the fumes from a 5%, freshly-prepared, aqueous solution of osmic acid (OsO4). This was followed by dehydration in ethyl alcohol and tertiary butyl alcohol, removal of air under vacuum and infiltration with paraffin.
Sections were cut 20 and 9Op thick and mounted with water.
Wax was removed by immersion in xylene. The sections were rehydrated in a series of ethyl alcohol dilutions, from concentrated to dilute, then transferred to distilled water.
Protein was then stained pink by immersion of the slides in an acidified 0.04% water solution of eosin Y, or starch was stained blue with a dilute aqueous solution of iodine. Ten grams iodine and 10 g. KI were dissolved in 25 ml. distilled water. This stock solution was diluted for use one to two hundred times.
The relationship between protein and starch was demonstrated by staining the sections with eosin, differentiating in 50% alcohol and staining with iodine.
When slides of cake crumb were prepared in this way, the fat was stained black, the protein bright pink and the starch granules a dark blue. 相似文献
Sections were cut 20 and 9Op thick and mounted with water.
Wax was removed by immersion in xylene. The sections were rehydrated in a series of ethyl alcohol dilutions, from concentrated to dilute, then transferred to distilled water.
Protein was then stained pink by immersion of the slides in an acidified 0.04% water solution of eosin Y, or starch was stained blue with a dilute aqueous solution of iodine. Ten grams iodine and 10 g. KI were dissolved in 25 ml. distilled water. This stock solution was diluted for use one to two hundred times.
The relationship between protein and starch was demonstrated by staining the sections with eosin, differentiating in 50% alcohol and staining with iodine.
When slides of cake crumb were prepared in this way, the fat was stained black, the protein bright pink and the starch granules a dark blue. 相似文献