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1.
Five distinct nuclear stains and staining procedures which utilize basic fuchsin as the dye have been studied, compared and tested on a Feulgen-weak fungus, Blastomyces dermatitidis, and other fungi.
Aqueous basic fuchsin has been shown to be an excellent, though impermanent, stain with which to study the nuclei of this and other fungi. The conditions under which formaldehyde acts as a mordant for basic fuchsin and produces a permanent nuclear stain have been established.
Comparison of crystal violet and basic fuchsin suggests that the mordanting action of the aldehyde operates through the para-amino groups of the dye. Certain other basic dyes were not mordanted by formaldehyde.
Gentle acid hydrolysis of the tissues has been found to be essential both to the specificity of the dye as a nuclear stain and to the mordanting effect of the aldehyde.
The possible relationship of these observations to the Feulgen reaction is discussed. A protocol for the method developed is presented. 相似文献
Aqueous basic fuchsin has been shown to be an excellent, though impermanent, stain with which to study the nuclei of this and other fungi. The conditions under which formaldehyde acts as a mordant for basic fuchsin and produces a permanent nuclear stain have been established.
Comparison of crystal violet and basic fuchsin suggests that the mordanting action of the aldehyde operates through the para-amino groups of the dye. Certain other basic dyes were not mordanted by formaldehyde.
Gentle acid hydrolysis of the tissues has been found to be essential both to the specificity of the dye as a nuclear stain and to the mordanting effect of the aldehyde.
The possible relationship of these observations to the Feulgen reaction is discussed. A protocol for the method developed is presented. 相似文献
2.
J. A. Rattenbury 《Biotechnic & histochemistry》1952,27(2):113-120
A method is described for staining nucleoli intensely by treating tissues with formaldehyde, hydrolysing in normal HC1 at 60°C. and staining with aceto-carmine. With correct hydrolysis time, chromosomes and cytoplasm are almost colorless.
Formaldehyde increases the acidity of cell parts, especially the nucleolus, presumably by neutralizing the basic protein groups, and increases the resistance to hydrolysis, perhaps by protecting the phospholipoprotein complexes which are most abundant in the nucleolus.
Hydrolysis reduces the acidity of cell parts, chiefly by removal of nucleic acids.
Aceto-carmine stains cell structures which are weakly acid in character (about pH 4-5) probably by precipitating as large dye aggregates.
The technic appears to be highly specific for nucleoli and related cell bodies. 相似文献
Formaldehyde increases the acidity of cell parts, especially the nucleolus, presumably by neutralizing the basic protein groups, and increases the resistance to hydrolysis, perhaps by protecting the phospholipoprotein complexes which are most abundant in the nucleolus.
Hydrolysis reduces the acidity of cell parts, chiefly by removal of nucleic acids.
Aceto-carmine stains cell structures which are weakly acid in character (about pH 4-5) probably by precipitating as large dye aggregates.
The technic appears to be highly specific for nucleoli and related cell bodies. 相似文献
3.
Methods are proposed for staining plant chromosomes with the dye brilliant cresyl blue, and for making these stained preparations permanent by using polyvinyl alcohol mounting medium.
The stain, which is composed of 2% brilliant cresyl blue in 45% aqueous acetic or propionic acid, is used with fixed material in making smear preparations. The technics for staining are similar to those employed in the aceto-carmine method.
The mounting medium is made by mixing 56% polyvinyl alcohol, which is diluted in water to the consistency of thick molasses, with 22% lactic acid and 22% phenol by volume. The permanent slides are made by floating off the cover slip of the temporary slide in 70% alcohol, then applying the mounting medium and replacing the cover slip.
The chief advantages of the methods described are:
1)The preparation of the stain is rapid and simple. The batch of stain will be good with the first try.
2)The staining procedure in some instances is shorter than when using aceto-carmine.
3)The stain shows a high degree of specificity for nuclear structures and gives better results than aceto-carmine when used on certain plant tissues.
4)A minimum number of cells is lost in making the slides permanent when using polyvinyl alcohol mounting medium as the slide and cover slip are run through only one solution prior to mounting.
5)The mounting medium dries rapidly and this shortens the time required before critical examination of the permanent mounts can be made. 相似文献
The stain, which is composed of 2% brilliant cresyl blue in 45% aqueous acetic or propionic acid, is used with fixed material in making smear preparations. The technics for staining are similar to those employed in the aceto-carmine method.
The mounting medium is made by mixing 56% polyvinyl alcohol, which is diluted in water to the consistency of thick molasses, with 22% lactic acid and 22% phenol by volume. The permanent slides are made by floating off the cover slip of the temporary slide in 70% alcohol, then applying the mounting medium and replacing the cover slip.
The chief advantages of the methods described are:
1)The preparation of the stain is rapid and simple. The batch of stain will be good with the first try.
2)The staining procedure in some instances is shorter than when using aceto-carmine.
3)The stain shows a high degree of specificity for nuclear structures and gives better results than aceto-carmine when used on certain plant tissues.
4)A minimum number of cells is lost in making the slides permanent when using polyvinyl alcohol mounting medium as the slide and cover slip are run through only one solution prior to mounting.
5)The mounting medium dries rapidly and this shortens the time required before critical examination of the permanent mounts can be made. 相似文献
4.
William B. Atkinson 《Biotechnic & histochemistry》1952,27(3):153-160
Some of the factors affecting the recoloration of Schiff's Reagent (fuchsin sulfurous acid or FSA) by formaldehyde have been studied spectrophotometrically to determine the optimal conditions for the reaction of this reagent with aldehydes.
Of the various reducing agents utilized in the preparation of the leuco dye from basic fuchsin, sodium sulfite and bisulfite proved to be the most satisfactory for obtaining in the reagent maximal sensitivity to recoloration with minimal quantitative variation of results.
The relative proportions of reducing agent and basic fuchsin present in die leuco dye determine its sensitivity to recoloration. Under the conditions of the present experiments, greatest reagent recoloration was obtained when the leuco dye contained 0.01 mole of sodium bisulfite and 0.001 mole of basic fuchsin per 100 ml., a ratio of 10/1.
The recoloration of a given amount of FSA is related to the amount of aldehyde and the temperature of the reaction.
The present experiments indicate the desirability of standardizing the composition of FSA and the conditions under which it is used, if the results of different investigators are to be readily reproduced or compared. 相似文献
Of the various reducing agents utilized in the preparation of the leuco dye from basic fuchsin, sodium sulfite and bisulfite proved to be the most satisfactory for obtaining in the reagent maximal sensitivity to recoloration with minimal quantitative variation of results.
The relative proportions of reducing agent and basic fuchsin present in die leuco dye determine its sensitivity to recoloration. Under the conditions of the present experiments, greatest reagent recoloration was obtained when the leuco dye contained 0.01 mole of sodium bisulfite and 0.001 mole of basic fuchsin per 100 ml., a ratio of 10/1.
The recoloration of a given amount of FSA is related to the amount of aldehyde and the temperature of the reaction.
The present experiments indicate the desirability of standardizing the composition of FSA and the conditions under which it is used, if the results of different investigators are to be readily reproduced or compared. 相似文献
5.
C. Nathaniel Wilson 《Biotechnic & histochemistry》1927,2(4):115-123
Several samples of neutral red have been studied; first, for the determination of their relative color intensities, and second, to determine their toxic effects on Paramoecium caudatum.
It was found that each of these dyes varied in physical characters both in dry form and in solution. The duration of life of groups of Paramoecia varied in each dye solution. These differences are probably due, at least in part, to differences in the chemical composition of each dye. This suggests that the varying results obtained by experimenters, in staining living material when using the same kind of dye under uniform conditions, may probably be attributed to these differences of chemical constitution of the dyes.
In the comparison of the toxic effects of the several samples most uniform results were obtained at concentrations of 1:5,000 and 1:10-000. At a concentration of 1:100,000 neutral red was found toxic but the results obtained were not in agreement with those obtained at lower concentrations. 相似文献
It was found that each of these dyes varied in physical characters both in dry form and in solution. The duration of life of groups of Paramoecia varied in each dye solution. These differences are probably due, at least in part, to differences in the chemical composition of each dye. This suggests that the varying results obtained by experimenters, in staining living material when using the same kind of dye under uniform conditions, may probably be attributed to these differences of chemical constitution of the dyes.
In the comparison of the toxic effects of the several samples most uniform results were obtained at concentrations of 1:5,000 and 1:10-000. At a concentration of 1:100,000 neutral red was found toxic but the results obtained were not in agreement with those obtained at lower concentrations. 相似文献
6.
Neutral red and the pyronins cannot be evaluated by means of reduction with titanous chloride, and market supplies of the stains contain nitrogenous dye intermediates which render other chemical methods of determining dye content unreliable.
Data are furnished in the present paper which will enable the analyst to obtain reliable dye-content values with samples of these dyes by means of a convenient spectrophotometric technic. 相似文献
Data are furnished in the present paper which will enable the analyst to obtain reliable dye-content values with samples of these dyes by means of a convenient spectrophotometric technic. 相似文献
7.
《Biotechnic & histochemistry》1944,19(3):119-122
DYES AND THEIR BIOLOGICAL USES Burckhalter, J. H., Jones, E. M., Holcomb, W. F., and Sweet, L. A. N-substituted 2-methoxy-6-chloro-9-aminoacridines. J. Amer. Chem. Soc., 65, 2012. 1943.
Galat, Alexander. New processes for sulfanilamide. Ind. and Eng. Chem., Ind. Ed., 36, 192. 1944.
Kumler, W. D., and Daniels, T. C. The relation between chemical structure and bacteriostatic activity of sulfanilamide type compounds. J. Amer. Chem. Soc., 65, 2190. 1943.
Kwartler, C. E., and Lucas, Philip. The preparation of sutfanil-amidoindazoles. J. Amer. Chem. Soc., 65, 1804. 1943.
Mueller, A. C., and Hamilton, C. S. The synthesis of 1-substituted aminobenzo(f)quinolines. J. Amer. Chem. Soc., 65, 1017. 1943.
Popkin, A. H. Derivatives of biphenylsulfonamides. I. Preparation of p-(o-aminopnenyl)-benzenesulfonamide. J. Amer. Chem. Soc., 65, 2043. 1943.
Popkin, A. H., and Perretta, Gertrude M. Derivatives of biphenyl-sulfonamide. II. Derivatives of p-(o-aminophenyl)-benzenesulfonamide. J. Amer. Chem. Soc., 65, 2046. 1943.
Shreve, R. N., and Bennett, R. B. Studies in azo dyes. I. Preparation and bacteriostatic properties of azo derivatives of 2,6-diaminopvridine. J. Amer. Chem. Soc., 65, 2241. 1943.
Shreve, R. N., and Bennett, R. B. Studies in azo dyes. II. Preparation and bacteriostatic properties of azo derivatives of 8-quinolino. J. Amer. Chem. Soc., 65, 2243. 1943.
Siebenmann, C., and Schnitzer, R. J. Chemotherapeutic study of p-nitrobenzoyl- and related compounds. J. Amer. Chem. Soc., 65, 2127 1943.
ANIMAL MICROTECHNIC Barrett, A. M. A method for staining sections of bone marrow. J. Path & Bact., 56, 133-5. 1944.
Barrett, A. M. On the removal of formaldehyde-produced precipitate from sections. J. Path. & Bact., 56, 135-6. 1944.
Chang, Min-Chueh. Disintegration of epidymal spermatozoa by application of ice to the scrotal testis. J. Exp. Biol., 20, 16-22. 1943.
Ercoli, N., and Lewis, M. N. The age factor in response of bone tissue to alizarin dyes and the mechanism of dye fixation. Anat. Rec., 87, 67-76. 1943.
Hess, Manfred, and Hollander, Franklin. Permanent metachromatic staining of gastric mucus smears. J. Lab. and Clin. Med., 29, 321-3. 1944.
Miller, John A. A new method of staining nervous tissue. Ohio J. of Sci., 44, 31-5. 1944. 相似文献
Galat, Alexander. New processes for sulfanilamide. Ind. and Eng. Chem., Ind. Ed., 36, 192. 1944.
Kumler, W. D., and Daniels, T. C. The relation between chemical structure and bacteriostatic activity of sulfanilamide type compounds. J. Amer. Chem. Soc., 65, 2190. 1943.
Kwartler, C. E., and Lucas, Philip. The preparation of sutfanil-amidoindazoles. J. Amer. Chem. Soc., 65, 1804. 1943.
Mueller, A. C., and Hamilton, C. S. The synthesis of 1-substituted aminobenzo(f)quinolines. J. Amer. Chem. Soc., 65, 1017. 1943.
Popkin, A. H. Derivatives of biphenylsulfonamides. I. Preparation of p-(o-aminopnenyl)-benzenesulfonamide. J. Amer. Chem. Soc., 65, 2043. 1943.
Popkin, A. H., and Perretta, Gertrude M. Derivatives of biphenyl-sulfonamide. II. Derivatives of p-(o-aminophenyl)-benzenesulfonamide. J. Amer. Chem. Soc., 65, 2046. 1943.
Shreve, R. N., and Bennett, R. B. Studies in azo dyes. I. Preparation and bacteriostatic properties of azo derivatives of 2,6-diaminopvridine. J. Amer. Chem. Soc., 65, 2241. 1943.
Shreve, R. N., and Bennett, R. B. Studies in azo dyes. II. Preparation and bacteriostatic properties of azo derivatives of 8-quinolino. J. Amer. Chem. Soc., 65, 2243. 1943.
Siebenmann, C., and Schnitzer, R. J. Chemotherapeutic study of p-nitrobenzoyl- and related compounds. J. Amer. Chem. Soc., 65, 2127 1943.
ANIMAL MICROTECHNIC Barrett, A. M. A method for staining sections of bone marrow. J. Path & Bact., 56, 133-5. 1944.
Barrett, A. M. On the removal of formaldehyde-produced precipitate from sections. J. Path. & Bact., 56, 135-6. 1944.
Chang, Min-Chueh. Disintegration of epidymal spermatozoa by application of ice to the scrotal testis. J. Exp. Biol., 20, 16-22. 1943.
Ercoli, N., and Lewis, M. N. The age factor in response of bone tissue to alizarin dyes and the mechanism of dye fixation. Anat. Rec., 87, 67-76. 1943.
Hess, Manfred, and Hollander, Franklin. Permanent metachromatic staining of gastric mucus smears. J. Lab. and Clin. Med., 29, 321-3. 1944.
Miller, John A. A new method of staining nervous tissue. Ohio J. of Sci., 44, 31-5. 1944. 相似文献
8.
Solubilities of dye-iodine precipitates in alcohol and in aqueous safranin solution were determined by direct solubility methods and by photocolorimetric methods. It was found that, increasing precipitate solubility in alcohol or safranin solution gave decreasing differentiation between Gram-positive and Gram-negative bacteria. Dyes which did not stain the cells well as a primary stain did not give good Gram stains, regardless of the solubilities of their precipitates. Some dyes (typified by methylene blue) which gave relatively alcohol-insoluble iodine precipitates gave inferior Gram differentiation because these precipitates were readily soluble in the safranin counterstain.
Solubilities of precipitates of crystal violet and various iodine substitutes were determined photocolorimetrically. The ability of a substance to replace iodine in the Gram stain correlated with its ability to give a precipitate which was only slightly soluble in alcohol and relatively insoluble in aqueous safranin solution.
It was concluded that the usual Gram reagents are not truly specific for the differentiation. Any dye and mordant could be used if the dye was deeply colored, stained the cells well, and if the precipitate of dye and mordant was only slightly soluble in alcohol and relatively insoluble in the counterstain. These factors, combined with those influencing differences in cell membrane permeability, constitute the most important factors in the Gram stain differentiation.
Studies were made concerning the ability of dyes to substitute for crystal violet in the Gram procedure. Of 29 dye samples reported on here for the first time none proved to be good substitutes for crystal violet. 相似文献
Solubilities of precipitates of crystal violet and various iodine substitutes were determined photocolorimetrically. The ability of a substance to replace iodine in the Gram stain correlated with its ability to give a precipitate which was only slightly soluble in alcohol and relatively insoluble in aqueous safranin solution.
It was concluded that the usual Gram reagents are not truly specific for the differentiation. Any dye and mordant could be used if the dye was deeply colored, stained the cells well, and if the precipitate of dye and mordant was only slightly soluble in alcohol and relatively insoluble in the counterstain. These factors, combined with those influencing differences in cell membrane permeability, constitute the most important factors in the Gram stain differentiation.
Studies were made concerning the ability of dyes to substitute for crystal violet in the Gram procedure. Of 29 dye samples reported on here for the first time none proved to be good substitutes for crystal violet. 相似文献
9.
H. A. Tobgy 《Biotechnic & histochemistry》1942,17(4):171-175
Root tips of Crepis species are fixed in La Cour's “2BE” and dehydrated thru a butyl alcohol series. They are stained in 1% crystal violet for 1 hour, with chromic acid and iodine as pre-and post-staining mordants, respectively, and passed thru dehydrating alcohols containing picric acid and ammonium hydroxide. Differentiation is done in clove oil. The method is rapid; the chromosomes are dark purple; the centromere is not stained; and the cytoplasm is clear. By further controlled destaining the hetero-chromatic segments within the chromosomes may be located.
Pollen mother cells are fixed in acetic alcohol (1:4) and squashed in aceto-carmine. A method is described for making semi-permanent preparations mounted in diaphane.
Pollen grains are mounted in lacto-phenol with acid fuchsin or anilin blue W. S. as the dye. 相似文献
Pollen mother cells are fixed in acetic alcohol (1:4) and squashed in aceto-carmine. A method is described for making semi-permanent preparations mounted in diaphane.
Pollen grains are mounted in lacto-phenol with acid fuchsin or anilin blue W. S. as the dye. 相似文献
10.
A method is described for the separation of azure A from commezcial samples of polychrome methylene blue. Up to 300 mg of the pure dye may be isolated in this way. The method is based on chromatography using columns 90 cm high, 7 cm in diameter, loaded with 3 g of polychrome methylene blue. The absorbent is silica gel, the eluent a mixture of acetic and formic acid.
Poor solubility of the dye acetate in water necessitates dissociation of the acetate by alkalinization and subsequent conversion of the dye to the chloride with diluted Ha. Demethylation that occasionally occurs during this procedure is negligible. Pure azure A does not spontaneously demethylate under ordinary conditions. 相似文献
Poor solubility of the dye acetate in water necessitates dissociation of the acetate by alkalinization and subsequent conversion of the dye to the chloride with diluted Ha. Demethylation that occasionally occurs during this procedure is negligible. Pure azure A does not spontaneously demethylate under ordinary conditions. 相似文献
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 E. Kindred 《Biotechnic & histochemistry》1935,10(1):7-20
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. 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
13.
Elizabeth F. Genung 《Biotechnic & histochemistry》1926,1(1):41-48
The writer has made an investigation of various samples of basic fuchsin for use in the Endo medium for differentiating the bacteria of the colon-typhoid group. Various different concentrations of the fuchsin samples have been used in making the media. The conclusions are as follows:
American made fuchsins differ markedly in their alcohol solubility properties. They contain materials which are very readily soluble in 95% alcohol, but which are precipitated by sodium sulphite.
This precipitation may be prevented by increasing the dilution of the fuchsin in alcohol.
In order to secure more dependable results in the use of decolorized basic fuchsin as an indicator in Endo Agar, it is advisable to test the fuchsin in different dilutions in alcohol in order to secure a completely decolorized solution. It is also advisable to carefully test those fuchsins which decolorize only in high dilutions with a known organism in Endo agar before relying on it as a satisfactory indicator for the presence of sewage organisms. 相似文献
American made fuchsins differ markedly in their alcohol solubility properties. They contain materials which are very readily soluble in 95% alcohol, but which are precipitated by sodium sulphite.
This precipitation may be prevented by increasing the dilution of the fuchsin in alcohol.
In order to secure more dependable results in the use of decolorized basic fuchsin as an indicator in Endo Agar, it is advisable to test the fuchsin in different dilutions in alcohol in order to secure a completely decolorized solution. It is also advisable to carefully test those fuchsins which decolorize only in high dilutions with a known organism in Endo agar before relying on it as a satisfactory indicator for the presence of sewage organisms. 相似文献
14.
-Chymotrypsin was immobilized on chitin from squills, lobsters and prawns by means of glutaraldehyde. Hydrolase and peptide synthetase activities were determined in aqueous and homogeneous aqueous-organic media, respectively.
The results show -chymotrypsin immobilized on chitin from prawn to be the most active immobilized derivative based on its synthetase activity (90% yield of Bz-Tyr-Leu-NH2 in carbonate buffer, pH 9 containing 70% 1,4- butanediol).
The relationship between the kinetic constant of hydrolysis and chitin structure was also studied. -Chymotrypsin immobilized on prawn chitin was found to be the best derivative in kinetic terms.
The stability of the three derivatives was studied at 37C. 相似文献
The results show -chymotrypsin immobilized on chitin from prawn to be the most active immobilized derivative based on its synthetase activity (90% yield of Bz-Tyr-Leu-NH2 in carbonate buffer, pH 9 containing 70% 1,4- butanediol).
The relationship between the kinetic constant of hydrolysis and chitin structure was also studied. -Chymotrypsin immobilized on prawn chitin was found to be the best derivative in kinetic terms.
The stability of the three derivatives was studied at 37C. 相似文献
15.
The phenyl and methyl trihydroxyfluorones, hitherto used histologically only in the rather difficult and unreliable Turchini tecbnics for discriminating deoxyribonucleic from ribonucleic acid, find a new use as iron mordant metachrome dyes which act as nuclear stains. Nuclear staining is unaffected by acid extraction of nudeic acids, as with hematoxylin lakes.
The two dyes, named by Liebermann and Lindenbanm 9-phenyl-2, 3, 7-trihydroxy-6-fluorone and 9-methyl-2, 3, 7-trihydroxy-6-Ruorone, have also acquired (illustrating with the phenyl homolog) longer chemical names of the form 2, 6, 7-trihydroxy-9-phenylisoxanthene-3-one (Eastman). Aldrich and Pfalz-Bauer adhere to the Liebermann-Lindenbaum nomenclature. The trivial name fluorone black is proposed for the phenyl homolog and methyl fluorone black for the methyl homolog.
The iron lake of fluorone black appears to be a useful substitute for iron hematoxylin, methyl fluorone black less useful. Neither dye has the diverse capability of hematoxylin.
Aided by a contract from the National Cancer Institute NO-1-CB-43912 相似文献
The two dyes, named by Liebermann and Lindenbanm 9-phenyl-2, 3, 7-trihydroxy-6-fluorone and 9-methyl-2, 3, 7-trihydroxy-6-Ruorone, have also acquired (illustrating with the phenyl homolog) longer chemical names of the form 2, 6, 7-trihydroxy-9-phenylisoxanthene-3-one (Eastman). Aldrich and Pfalz-Bauer adhere to the Liebermann-Lindenbaum nomenclature. The trivial name fluorone black is proposed for the phenyl homolog and methyl fluorone black for the methyl homolog.
The iron lake of fluorone black appears to be a useful substitute for iron hematoxylin, methyl fluorone black less useful. Neither dye has the diverse capability of hematoxylin.
Aided by a contract from the National Cancer Institute NO-1-CB-43912 相似文献
16.
Chromatographic analysis of commercial batches of toluidine blue shows these to be dye mixtures. Histologically, some samples were found to be poor metachromatic dyes. These unsatisfactory stains contained blue dyes with little or no metachromatic properties as well as a metachromatic fraction. On the other hand, contaminating dyes in histologically satisfactory samples had poor staining qualities and hence did not interfere with the color produced by the metachromatic fraction.
Chromatographic fractionation of different commercial batches of toluidine blue yielded identical, homogeneous metachromatic dyes. These purified dyes had a peak absorption at 615 mμ in contrast to that of purified azure A whose peak absorption was at 622.5 mμ. 相似文献
Chromatographic fractionation of different commercial batches of toluidine blue yielded identical, homogeneous metachromatic dyes. These purified dyes had a peak absorption at 615 mμ in contrast to that of purified azure A whose peak absorption was at 622.5 mμ. 相似文献
17.
Lydi Sterrenberg Rinette H. M. Julicher Peter A. L. Goossens Aalt Bast Jan Noordhoek 《Free radical research》1986,1(6):369-378
The stimulation of non-enzymic lipid peroxidation by doxorubicin, daunorubicin and 7 derivatives was investigated in extracted microsomal phospholipids and in intact microsomes.
Evidence was obtained for the necessity of a free amino-sugar moiety for a stimulative effect on lipid peroxidation. Binding of anthracyclines to RNA (which is present in microsomes) was inhibitory towards stimulation.
Drugs that stimulated lipid peroxidation in a non-enzymic system with extracted phospholipids also were stimulative in an enzymic, NADPH-dependent, microsomal system. They were not always effective in intact microsomes without the enzymic system.
The role of the enzymic system in the stimulation of anthracycline induced lipid peroxidation is thought to be the reduction of iron ions rather than the stimulation of oxygen radical production via the anthracyclines. 相似文献
Evidence was obtained for the necessity of a free amino-sugar moiety for a stimulative effect on lipid peroxidation. Binding of anthracyclines to RNA (which is present in microsomes) was inhibitory towards stimulation.
Drugs that stimulated lipid peroxidation in a non-enzymic system with extracted phospholipids also were stimulative in an enzymic, NADPH-dependent, microsomal system. They were not always effective in intact microsomes without the enzymic system.
The role of the enzymic system in the stimulation of anthracycline induced lipid peroxidation is thought to be the reduction of iron ions rather than the stimulation of oxygen radical production via the anthracyclines. 相似文献
18.
A simple and rapid method for the simultaneous quantitative analysis of mixtures of hematoxylin and hematein uses the molar extinction coefficients of the pure substances calculated by Lalor and Martin (1959). Absorbance measurements of the samples dissolved in methanol are made at wavelengths of 292 nm and 445 nm, the wavelengths of maximum absorption of hematoxylin and hematein respectively. The hematoxylin absorbance at 292 nm is corrected for the presence of hematein.
Using this method it was found that of 12 commercial samples labelled “hematoxylin” all contained at least 90% of the compound. Hematein contents of these samples fell in the range 0.1% to 6.8%. In 9 commercial samples labelled “hematein” the hematein contents fell in the range 1.2% to 90.7%. The hematoxylin contents of these samples fell in the range of 1.0% to 82.7%.
This paper describes also a chromatographic method for the identification of hematein and its oxidation products. 相似文献
Using this method it was found that of 12 commercial samples labelled “hematoxylin” all contained at least 90% of the compound. Hematein contents of these samples fell in the range 0.1% to 6.8%. In 9 commercial samples labelled “hematein” the hematein contents fell in the range 1.2% to 90.7%. The hematoxylin contents of these samples fell in the range of 1.0% to 82.7%.
This paper describes also a chromatographic method for the identification of hematein and its oxidation products. 相似文献
19.
Elizabeth F. Genung 《Biotechnic & histochemistry》1926,1(4):135-142
In describing a method of testing for the return of color in decolorized fuchsin for use in Endo Medium, French states that variations in hydrogen ion concentration fail to influence the appearance of color in this medium.
Duplications of this test were made using alcoholic and aqueous solutions of fuchsin and both sodium sulfite and sodium bisulfite as decolorizing agents.
In the decolorized alcoholic solutions of fuchsin the color failed to reappear when formalin was added, but a small amount of a weak solution of lactic acid caused the color to return.
Alcoholic solutions of fuchsin failed to decolorize in sodium bisulfite solutions until a few drops of NaOH were added. The color, then, reappeared immediately.
Solutions of peptones to which fuchsin had been added were substituted for the original fuchsin solution. Alcoholic and aqueous solutions of fuchsin were added to equal amounts of a 1% peptone solution. The peptone solutions varied in their hydrogen ion concentration and the results showed that those which were neutral decolorized readily while the more acid solutions were but partially decolorized.
Fuchsin decolorized according to results found in this test, was not satisfactory in the Endo medium, especially in the case of the aqueous solutions of fuchsin.
Experiments which were carried on by other workers and checked with this method all indicated that some acid is necessary to secure the restoration of color. 相似文献
Duplications of this test were made using alcoholic and aqueous solutions of fuchsin and both sodium sulfite and sodium bisulfite as decolorizing agents.
In the decolorized alcoholic solutions of fuchsin the color failed to reappear when formalin was added, but a small amount of a weak solution of lactic acid caused the color to return.
Alcoholic solutions of fuchsin failed to decolorize in sodium bisulfite solutions until a few drops of NaOH were added. The color, then, reappeared immediately.
Solutions of peptones to which fuchsin had been added were substituted for the original fuchsin solution. Alcoholic and aqueous solutions of fuchsin were added to equal amounts of a 1% peptone solution. The peptone solutions varied in their hydrogen ion concentration and the results showed that those which were neutral decolorized readily while the more acid solutions were but partially decolorized.
Fuchsin decolorized according to results found in this test, was not satisfactory in the Endo medium, especially in the case of the aqueous solutions of fuchsin.
Experiments which were carried on by other workers and checked with this method all indicated that some acid is necessary to secure the restoration of color. 相似文献
20.
This paper shows that by using solutions heated in the incubator during certain stages, the alizarin red S method of staining the ossified centers in embryos has been shortened, with a consequent saving in time.
New methods of mounting the specimens have been evolved and are described in detail.
The technic of photographing mounted and unmounted specimens is outlined and illustrated by diagrams.
Diagrammatic illustrations are provided of the various types of apparatus used, including a plan of the cabinet for demonstrating clearly the smaller embryos mounted between watch glasses. Photographic examples of the results achieved are also shown. 相似文献
New methods of mounting the specimens have been evolved and are described in detail.
The technic of photographing mounted and unmounted specimens is outlined and illustrated by diagrams.
Diagrammatic illustrations are provided of the various types of apparatus used, including a plan of the cabinet for demonstrating clearly the smaller embryos mounted between watch glasses. Photographic examples of the results achieved are also shown. 相似文献