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1.
For a detailed study of chromosome morphology in meiotic prophase stages of Beta species, a special double staining technic has been developed. It consists of combined maceration-staining in an ethanol-hydrochloric acid-carmine mixture followed by poststaining of the squashed material in a diluted Giemsa solution. The technic yields well-spread prophase meiotic nuclei showing detailed structures both in weaker stained chromosome segments and in threadlike chromatin structures. This technic proved to be especially favorable for stages which are difficult to interpret, such as pachytene, schizotene and diffuse stages.  相似文献   

2.
For a detailed study of chromosome morphology in meiotic prophase stages of Beta species, a special double staining technic has been developed. It consists of combined maceration-staining in an ethanol-hydrochloric acid-carmine mixture followed by poststaining of the squashed material in a diluted Giemsa solution. The technic yields well-spread prophase meiotic nuclei showing detailed structures both in weaker stained chromosome segments and in threadlike chromatin structures. This technic proved to be especially favorable for stages which are difficult to interpret, such as pachytene, schizotene and diffuse stages.  相似文献   

3.
The Feulgen technic as modified by Heitz promises to become an extremely useful tool in the solution of certain cytological problems. A procedure is outlined for using this technic with root tip smears, and smears of plant microspores. The chief improvement suggested over previous methods is that the material be mounted in euparal, after immersion in 95% alcohol. The technic is of value in the study of chromosome fragmentation, chromatid coiling, centromeres, etc., in both somatic tissue and in microspores.  相似文献   

4.
The combined alcian blue (AB)/PAS technic is widely used for the detection and characterization of mucosubstances in tissue sections. Mostly the sequence AB/PAS is used, occasionally also the reserved sequence PAS/AB. The present study shows clearly that the sequence of the combined technic, i.e. AB/PAS or PAS/AB is substantially influencing the results. So it could be demonstrated that by using the combination PAS/AB originally PAS-positive and AB-negative reacting mucosubstances become AB-positive. This could be caused by periodic acid oxidation followed by addition of hydrogen sulfite to aldehyde group thus providing secondary basophilic resp. AB positive material.  相似文献   

5.
Summary The combined alcian blue (AB)/PAS technic is widely used for the detection and characterization of mucosubstances in tissue sections. Mostly the sequence AB/PAS is used, occasionally also the reserved sequence PAS/AB. The present study shows clearly that the sequence of the combined technic, i.e. AB/PAS or PAS/AB is substantially influencing the results. So it could be demonstrated that by using the combination PAS/AB originally PAS-positive and AB-negative reacting mucosubstances become AB-posltive. This could be caused by periodic acid oxidation followed by addition of hydrogen sulfite to aldehyde group thus providing secondary basophilic resp. AB positive material.  相似文献   

6.
We report 23 cases of small supernumerary chromosome examined at the Medical Genetics Center of Marseille. Genetic counselling is depending on the origin of the additional chromosomal material. Among the different cytogenetic technics which are useful in such an identification in situ hybridisation is a new technic very helpful in some cases, especially iso p18.  相似文献   

7.
A chemical and histochemical study of Gomori's acid phosphatase technic showed that the causes of its unreliability were: (1) that fixation and other steps of histological procedure inactivate the enzyme to a great extent; (2) the enzyme may diffuse, as demonstrated in frozen sections of acetone-fixed material; and (3) some absorption of lead by the sections takes place. Much of this unreliability is avoided, however, by maintaining as low a temperature as possible during fixation and dehydration, with exposure to the temperature of the paraffin oven for the shortest possible length of time. The relative insolubility and thermo-stability of the enzyme, moreover, indicate the possibility of devising a more satisfactory technic in the future.  相似文献   

8.
A statement is given of the advantages of this special technic and its place in embryological investigations, including directions for selecting the proper stages in collecting conifer cones and ovules, their methods of dissection from living material and their preservation for later dissection. The choice of dissecting microscopes and dissecting instruments, as well as directions for staining embryos with phloxine which may be combined with slow dehydration in glycerin, or for staining with Delafield's or Heidenhain's hematoxylin which may be followed by the glycerin dehydration are described. Glycerin affords a convenient break for a temporary stopping place in this technic.

Directions are given for transfer from glycerin thru 95% and absolute ethyl alcohol into other solvents such as diaphane solvent, essence of euparel or an easily prepared sandarac solvent. Other mounting media which have been used for conifer embryos are discussed—glycerin jelly, Venetian turpentine and Canada balsam—emphasizing the special advantages found in the media employing sandarac.  相似文献   

9.
SYNOPSIS. Activities of sheep coccidia in stages of in vitro excystation, and of Eimeria tenella removed in stages of excystation from the chicken were arrested by lowering the temperature of the parasites; in a cooled condition, the parasites remained apparently unchanged for at least 1-2 days. When transferred later to the warming stage of the microscope, they quickly resumed excystation. A cold storage technic for E. tenella was developed. The technic might also help in studying other gastrointestinal parasites and might also provide material for classroom work.  相似文献   

10.
A technic is outlined for the preparation of difficult material for the study of chromosome number and morphology in root-tip smears. The chief objective is to obtain polar views of the metaphase plates rather than equatorial views. To achieve this end it is recommended that fresh root-tips be cut free-hand into thin cross sections. The important features are: thin freehand cross sectioning of the fresh root-tips; fixing in Belling's iron aceto-carmine solution; maceration for 2-5 minutes in 50% HCl in 95% alcohol; and mounting in “Diaphane.”  相似文献   

11.
Using a buffered acid thionin stain with carbolxylene as a clearing agent, a reliable stain for Nissl bodies may be performed on frozen sections of fresh or old formalin-fixed material in a relatively short period of time. The technic is simple: the buffering of thionin makes regressive differentiation unnecessary.  相似文献   

12.
Summary Previous histochemical investigations demonstrated similarities in the binding of Congo Red and other direct cotton dyes by amyloid and cellulose. It seemed threfore of interest to determine whether or not the cellulose-like reactivity of amyloid extends also to dye solutions containing an anionic reserving agent. These reagents are used in the dyeing of wool-cellulose (Halbwolle) fabrics to prevent binding of direct cotton dyes by proteins. Mesitol WLS-Congo Red solutions stained amyloid selectively; other tissue structures, except some hyaline deposits in arterioles, remained unstained. The cause of this non-specific reaction could not be determined with certainty. Therefore, the alkaline Congo Red method is recommended for histochemical identification of amyloid. However, the Mesitol WLS-Congo Red technic was very useful for demonstration of amyloid after prolonged storage of tissues in formalin; amyloid in such material showed little or no reactivity with the alkaline Congo Red or the Sirius dye methods. This pilot study indicates that anionic reserving agents can be effectively employed under conditions of histochemical technics.  相似文献   

13.
The technic described involves the use of a saturated solution of picric acid in absolute alcohol in the process of dehydration following the gentian-violet-iodine stain as applied to plant cytological material. The method is suitable for both paraffin sections and smears of pollen mother cells fixed in Navashin's or Flemming's solutions. Differentiation in clove oil is very easy since cytoplasm destains immediately, while chromatic material destains very slowly following picric acid. Chromosomes are stained more distinctly than with the usual Gram stain and do not fade.  相似文献   

14.
The effect of oxidation on neurofibrillar argyrophilia was studied by subjecting nervous tissues containing both normal and degenerating fibers to the action of potassium permanganate, periodic acid, chromic acid, lead tetraacetate, and sodium bismuthate prior to silver impregnation. The argyrophilic response of normal fibers to such treatment was studied with the Nonidez silver nitrate block technic, the double impregnation method of Bielschowsky on both blocks and sections, and a silver proteinate procedure. The response of degenerating fibers was studied by the Cajal formula 6 block technic and the modified Bielschowsky procedure of Nauta and Ryan for sections. The experimental data indicated that such oxidation did not produce any differential staining effects between normal or degenerating fibers.  相似文献   

15.
It has been found that a plastic spray (“Krylon”, manufactured by Krylon, Inc., 2601 Broad Street, Philadelphia, Pa.) is suitable as a covering medium for stained, paraffin-embedded tissue sections. The material is supplied in an aerosol bomb type dispenser. The technic and advantages of using a plastic spray to replace both the usual mounting medium and cover glass are described below.  相似文献   

16.
Cannulation of the aorta of the mouse through an incision in the left ventricle has permitted the introduction of various injection media into the arterial tree. Heparinized mice, sacrificed by ether, were exsanguinated and injected with latex, latex-thorotrast or vinyl acetate. The apparatus consists of a special cannula made by combining a 1 inch segment of a 23 gauge hypodermic needle and fine polyethylene tubing (PE 50, intramedic). Nearly all of the vascular tree was injected with this technic. Latex-thorotrast injections have the decided advantage of permitting combined X-ray and histologic study of the material. The procedure was devised in the course of an attempt to evaluate the relationship between circulatory changes and experimentally produced bone absorption and new bone formation in mice.  相似文献   

17.
To study chromosomes in bull testes and their behavior at meiosis, a prefixation treatment with hypotonic solutions was used. After fixation, the material was squashed and stained with Feulgen's nucleal reaction. When needed, additional staining with iron-hematoxylin was feasible. The hypotonic Tyrode solutions of 10 to 20% normal strength were prepared according to A. Hughes (1952); the time of pretreatment was, in general, 15-30 min; fixation was made in glacial acetic acid-absolute alcohol (1:3) and Feulgen squash technic was carried out according to Schedule 5 of Darlington and La Cour (1947). Morphologic details were well preserved and photomicrographs of well-spread chromosomes in one plane were obtained easily.  相似文献   

18.
The authors present a new technic to point out the rheumatoid factor by immunofluorescence and compare this technic and the others to classical technics of agglutination. This technic allows to avoid the absorption of rheumatoid factor in the serological reactions using the immunofluorescence.  相似文献   

19.
To simplify the staining of animal chromosomes (especially in insect testes) the authors have borrowed (with necessary modifications) the squash technic of plant cytology. The method has four steps: (1) Water pretreatment. This step requires only about 5-10 minutes either in water at room temperature or in water kept at about 38°C. in a water bath. (2) Fixation. Ordinarily only 5 minutes in 10-15% aqueous solution of glacial acetic acid is necessary. (3) Staining. The fixed tissue is rinsed in two or three changes of distilled water and then placed in a solution of basic fuchsin: either 1% in 30% ethyl alcohol, or 0.2-0.4% in 5-10% lactic acid. In the former solution the staining period should be about 2 minutes: in the latter, 5-20 minutes. The time is not critical. (4) Squashing. The material is rinsed in several changes of distilled water, placed on a clean slide and squashed under a cover glass. Such preparations last 4-5 weeks, and a technic is described for removing the cover glass in order to mount in Euparal and to make them permanent. The authors list various species of vertebrates as well as invertebrates in which the technic has given good chromosome staining, as shown by illustrations.  相似文献   

20.
A brief review is given of some of the older technics of clearing and staining various types of animals, in such a way that the bones are clearly visible in the surrounding tissues. The authors have modified some of these earlier practices. Particularly good results were obtained by combining the Schultze technic with that of Lundvall. Embryos are fixed in 95% alcohol, treated with 1% KOH, stained in 1:10,000 alizarin Red S, cleared in gylcerin, dehydrated with alcohol and further cleared in toluol, toluol saturated with naphthalene, and anise oil saturated with naphthalene. Details of the technic are presented in the text  相似文献   

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