The preparation of microtome sections of unaltered soil for the study of soil organisms in situ

Summary A new technique for study of small soil organisms in situ in unaltered soil is described.The soil samples are cooled in a refrigerator at — 10°C to kill the animals. A small portion taken from a frozen soil sample, is slowly immersed in a solution of gelatin. When the specimen is infiltrated with gelatin and the whole cooled it is fixed in formalin to enable it to withstand treatment with hydro-fluoric acid for removal of sand grains. Subsequently the specimens are immersed in gelatin solution for a second time after which the specimens are affixed to wooden blocks which can be clamped in the microtome. Before sectioning, the embedded specimen affixed to the wooden block is hardened in methylalcohol after which it is possible to cut sections 7,5–10µ thick.The most satisfactory staining procedure proved to be the quadruple staining method of Johansen. By this method nematodes, fungi, bacteria and amoebae are easily distinguishable from the soil particles.     

Accurate Placement of Ultrathin Sections on Grids; Control by Sol-Gel Phases of a Gelatin Flotation Fluid

A 3% solution of gelatin in a petri dish at 25-30 C. provides a liquid, viscous surface upon which ultrathin sections can be floated. On cooling, the gelled substratum immobilizes the sections, allowing grids to be placed on them with any desired grid-to-section orientation. When the gelatin is remelted, the sections remain attached to the grids. After draining, traces of gelatin adhering to the grids are removed by flotation (section side down) for 30 min on 2% acetic acid at 60 C. This is followed by flotation for 3-5 min on Tris buffer, pH 7.1, and then on distilled water for 30 min—both treatments at 60 C. The technique is particularly useful for mounting serial sections.     

N-butyl Methacrylate and Paraffin as an Embedding Medium for Light Microscopy

A method of tissue embedding using n-butyl methacrylate and paraffin is described. Following alcohol dehydration and infiltration with the methacrylate monomer, tissues are embedded in gelatin capsules in a mixture consisting of 3.5 g of paraffin for each 10 ml of methacrylate. Benzoyl peroxide (0.2 g for each 10 ml of monomer) is added as the catalyst and the methacrylate polymerized in a 50 C oven for 18-24 h. Following polymerization the block is trimmed and embedded in paraffin to provide a firm support during sectioning. A water trough attached to the microtome knife is essential to facilitate the handling of sections and ribbons. For serial sections a mixture of equal weights of beeswax and paraffin is used to make the sections adhere to each other. Usual staining procedures can be used since the embedding medium is readily soluble in xylene.     

N-Butyl methacrylate and paraffin as an embedding medium for light microscopy.

A method of tissue embedding using n-butyl methacrylate and paraffin is described. Following alcohol dehydration and infiltration with the methacrylate monomer, tissues are embedded in gelatin capsules in a mixture consisting of 3.5 g of paraffin for each 10 ml of methacrylate. Benzoyl peroxide (0.2 g for each 10 ml of monomer) is added as the catalyst and the methacrylate polymerized in a 50 C oven for 18--24 h. Following polymerization the block is trimmed and embedded in paraffin to provide a firm support during sectioning. A water trough attached to the microtome knife is essential to facilitate the handling of sections and ribbons. For serial sections a mixture of equal weights of beeswax and paraffin is used to make the sections adhere to each other. Usual staining procedures can be used since the embedding medium is readily soluble in xylene.     

Ultrasound-guided fetal intravenous transfusion for severe rhesus haemolytic disease.

Intrauterine, intraperitoneal transfusion is associated with a poor survival rate in fetuses with hydrops and low gestational age. A method of direct fetal intravenous transfusion was used in two fetuses. One fetus with severe rhesus haemolytic disease was given transfusions in the 29th and 30th weeks of gestation, using an ultrasound-guided needle through the hepatic part of the umbilical vein without fetoscopy. In another fetus, an experimental cannulation of the umbilical vein succeeded in the 23rd week of gestation. Ultrasound-guided fetal intravenous transfusion avoids the use of fetoscopy, which has limitations, and may improve the prognosis for rhesus-sensitised fetuses.     

A Sudan Black B Myelin Stain for Peripheral Nerves

Blocks of fresh issue were fixed 2 or more days in: cobalt sulfate (or nitrate), 1 gm; distilled water, 80 ml; 10% calcium chloride, 10 ml; and formalin, 10 ml. The fixed tissue was washed thoroughly in tap water, embedded in gelatin, frozen sections cut, and mounted on slides with gelatin adhesive. The sections were stained 15-30 min in a saturated, filtered solution of Sudan black B in 70% alcohol, differentiated in 50% alcohol under microscopic observation, and a cover glass applied with glycerol-gelatin. In thick (50-100 μ) sections, myelin stained green to gray-green and this allowed easy differentiation between nerves and other tissue elements.     

Teratogenic effects of nicotine on palate formation in mice

Fetuses of pregnant CD-1 mice, exposed to intraperitoneal injection of 0.1% nicotine sulfate at a dose of 1.67 mg/kg body weight/day on gestational days 6-15, were compared with control (saline injected and non-injected) fetuses to assess the effects of nicotine on fetal growth in general and palatogenesis in particular. A total of 59 pregnant females (18 experimental and 41 control) were sacrificed on the 18 th gestational day and their fetuses were examined gross morphologically and histologically (using serial sections through the head in the frontal plane). Data analysis revealed that maternal weight gain, crown-rump length, fetal weight and head dimensions were significantly reduced in nicoted treated animals when compared to those of the controls. Histological examination revealed that 9.6% of fetuses of nicotine injected mothers presented clefts of the palate, whereas none of the control fetuses had that anomaly. It was concluded that nicotine has a detrimental effect on general growth and development as well as on palatogenesis of mice.     

A simple method of staining juxtaglomerular granules in the rat kidney for high resolution light microscopy

A simple method for the demonstration of juxtaglomerular granules in Epon embedded semithin (0.5-1 micrometer) sections has been developed as follows: sections are prepared as for routine electron microscopy except that before dehydration, the tissues are immersed in 0.5% uranyl acetate in Veronal acetate buffer (pH 5.0) overnight at room temperature. After sectioning on an ultramicrotome, the semithin sections are briefly stained with toluidine blue-pyronin Y. After staining, the section is rinsed in running tap water and then air dried. Under a light microscope with a 40 X or a 100 X objective, the juxtaglomerular granules appear as deep purple particles and are thus easily separated from the bluish cytoplasm of the juxtaglomerular cells. Cellular organelles in other cells of the kidney were also clearly stained and their fine structure distinguishable.     

Gestational changes in concentrations of selenium and zinc in the porcine fetus and the effects of maternal intake of selenium

The effect of maternal dietary selenium (Se) and gestation on the concentrations of Se and zinc (Zn) in the porcine fetus were determined. Mature gilts were randomly assigned to treatments of either adequate (0.39 ppm Se) or low (0.05 ppm Se) dietary Se. Gilts were bred and fetuses were collected throughout gestation. Concentrations of Se in maternal whole blood and liver decreased during gestation in sows fed the low-Se diet compared to sows fed the Se-supplemented diet. Maternal intake of Se did not affect the concentration of Se in the whole fetus; however, the concentration of Se in fetal liver was decreased in fetuses of sows fed the low-Se diet. Although fetal liver Se decreased in both treatments as gestation progressed, the decrease was greater in liver of fetuses from sows fed the low-Se diet. Dietary Se did not affect concentrations of Zn in maternal whole blood or liver or in the whole fetus and fetal liver. The concentration of Se in fetal liver was lower but the concentration of Zn was greater than in maternal liver when sows were fed the adequate Se diet. These results indicate that maternal intake of Se affects fetal liver Se and newborn piglets have lower liver Se concentrations compared to their dams, regardless of the Se intake of sows during gestation. Thus, the piglet is more susceptible Se deficiency than the sow.     

Bulk Handling Racks for Free-Floating Serial Sections, Especially Suitable for Nauta Staining

Staining racks, each containing 20 shallow compartments, were constructed by drilling 1.5 cm holes in 8 × 11 cm sheets of 1 mm thick Darvic, an unplasticised polyvinyl-chloride compound, and cementing fibre-glass gauze of 1.3 mm mesh size to one surface. Sections were placed serially—one to each compartment—in the racks, and stacks of up to 9 racks were clamped by Perspex (methyl methacrylate) nuts and bolts, and side clamps. Thus, sections could be handled easily and kept in strict serial order, even in bulk. For Nauta staining, brains had to be gelatin embedded before sectioning. By storing sections in groups of 4 in ice-cube trays, evenly spaced series could be selected for placement in the racks. As many as 160 sections were taken together through all stages of the Nauta method, the timing of critical stages being controlled by taking 4 to 6 free-floating sections, together with the racks, through the various solutions.     

A Simple Method of Staining Juxtaglomerular Granules in the Rat Kidney for High Resolution Light Microscopy

A simple method for the demonstration of juxtaglomerular granules in Epon embedded semithin (0.5-1 μm) sections has been developed as follows: sections are prepared as for routine electron microscopy except that before dehydration, the tissues are immersed in 0.5% uranyl acetate in Veronal acetate buffer (pH 5.0) overnight at room temperature. After sectioning on an ultramicro-tome, the semithin sections are briefly stained with toluidine blue-pyronin Y. After staining, the section is rinsed in running tap water and then air dried. Under a light microscope with a 40 × or a 100 × objective, the juxtaglomerular granules appear as deep purple particles and are thus easily separated from the bluish cytoplasm of the juxtaglomerular cells. Cellular organelles in other cells of the kidney were also clearly stained and their fine structure distinguishable.     

Improved Sectioning and Berlin Blue Staining of Whole Human Brain

Brain sectioning has been improved through gelatin embedding so that more than forty precisely oriented serial sections can be obtained from a single brain. Since the embedding gelatin requires no fixation, it can be removed from the sections prior to staining by simple warming. The reduction of Berlin blue dye commonly observed after staining by the Mulligan method has been found to be at least partly due to light in the UV to near UV range. Dye reduction is significantly inhibited by postfixation in 25% acetic acid.     

Improved sectioning and Berlin blue staining of whole human brain

Brain sectioning has been improved through gelatin embedding so that more than forty precisely oriented serial sections can be obtained from a single brain. Since the embedding gelatin requires no fixation, it can be removed from the sections prior to staining by simple warming. The reduction of Berlin blue dye commonly observed after staining by the Mulligan method has been found to be at least partly due to light in the UV to near UV range. Dye reduction is significantly inhibited by postfixation in 25% acetic acid.     

Lead acetate as a vital marker for the analysis of bone growth

The use of lead acetate as a vital stain adds another method for the study of periodic appositional patterns of hard tissues. The distinct advantage of this technique is that these tissues can be decalcified and examined histologically without loss of the marker. The following method was used in preparation of the sections shown in the text. The rats received an intravenous injection of 4 mg lead acetate/kg body weight. After sacrifice, the tissues were decalcified in 1% HCL through which H₂S was constantly bubbled. The action of the H₂S gas is to convert the lead at sites of calcification to insoluble lead sulfide. Upon completion of decalcification the sections were embedded in 30% gelatin, and frozen sections at 15–20 μ were cut. The sections were then placed in a 0.1% solution of gold chloride for ten minutes. Next, they were placed in a 5% solution of sodium bisulphate for ten minutes. Subsequently they were washed in distilled water for 30 minutes and finally fixed in a 5% solution of sodium thiosulphate. No additional staining was used. The sections were then mounted with glycerine jelly. The resulting lead lines are sharp and therefore conducive to quantitative measurements. Because of the relatively thin sections cut, histologic details can be observed.     

Zinc Chromate Modification of the Golgi Technic

A modification of the Golgi technic is described in which the reaction takes place in well fixed formalin material. Thin slices (whole sections of adult monkey, cat and rat cerebrum) 2 to 3 mm. thick, from brains fixed 3 to 4 months in 10% formalin, are chromated for two days in 3 g. of zinc chromate dissolved in 98 ml. of distilled water and 2 ml. of formic acid. Slices are then removed, blotted dry and immersed, suspended by a thread, in 0.75% silver nitrate solution for two days. Solution should be changed after the first day. After silvering, the slices are dehydrated rapidly (total time about one hour) in 95% and absolute alcohol, placed in xylene 10 minutes, in low melting point paraffin 10 minutes and embedded in low melting point paraffin. Only surface infiltration is necessary since sections are cut 90 to 100 u. Sections are collected in 95% alcohol, dehydrated in absolute alcohol, cleared in several changes of xylene and mounted in Fisher's Permount. Results with fetal and new born material were not good.     

Affixing Polyester Wax Sections to Glass Slides by Celloidin and Cellulose Acetate Applied in Sequence

Sections cut from material embedded in polyester wax can be firmly attached as follows: One drop of a 2% solution of celloidin in amyl acetate is smeared on clean slides, and sections taken from the floatation water onto these slides are dried at room temperature. After drying the slides are immersed in a 2% solution of cellulose acetate in acetone for 1 min, transferred directly to absolute ethanol, through 50% ethanol, and into water. Sections affixed by this method and stained by either hematoxylin-eosin or toluidine blue schedules do not loosen and have negligible background staining.     

Form and development of the human fetal subarachnoid cistern]

The development and form of the human fetal subarachnoid spaces have been elucidated by reconstruction (34 mm CRL fetus) and by plastic casts (several 20-30 cm CRL fetuses). Equivalents of adult cisterns are present in the young fetus. In older fetuses the cisternal shape is of adult type. It is suggested that pressure from the growing brain produces tension in the arachnoid mesenchyme and determines the initial orientation of the endo-ecto-meningeal limiting membrane. The fluid-filled subarachnoid spaces and the fetal brain together form a composite structural unit probably defining the configuration of the fetal head capsule. Prospective sutures develop over the inner ridges of the fetal dura. However, the lambda suture and the associated base of the tentorium eventually separate.     

The Benzidine Staining Method for Blood Vessels

Two modifications of the method are described: A. Living specimens of sabellid and serpluid polychaetes, earthworms, small tadpoles, or fish larvae are immersed in an approximately saturated solution of benzidine for 30 minutes and then 3% hydrogen peroxide is added until bubbles of gas appear. When the blood vessels appear dark blue, the specimens are fixed in acidified 70% alcohol, dehydrated, cleared and either mounted in Canada balsam as whole mounts, or embedded in paraffin, sectioned at 100 to 250µ and mounted. B. Material fixed in 10% formalin in sea-water, or in formalin hypertonic saline, is incubated at 37°C. for one hour in an aqueous mixture containing sodium nitroprusside, 0.1%; benzidine, acetic acid 0.5%, followed by a weak (0.01–0.02%) hydrogen peroxide solution for a further hour, embedded in paraffin, cut into thick sections and mounted.     

The renal response to the ingestion of fluid by the fetal sheep

To see if the variability in fetal urine flow and sodium excretion was related to fetal drinking activity, renal function was investigated in two groups of oesophageally-ligated fetuses and one group of non-ligated fetuses. There was no significant difference in urine flow, sodium excretion or glomerular filtration rate in the ligated fetuses compared with the non-ligated fetuses. Furthermore, oesophageal ligation had no effect on the variability in urine flow and sodium excretion rate. The response of fetal kidney to ingestion of fluid was investigaeed in 2 groups of oesophageally-ligated fetuses. In one group it was shown that ingestion of 20 ml/kg of amniotic fluid by the fetus had no consistent effect on fetal renal function. In the other group it was shown that the ingestion of 200 ml water also had no consistent effect on fetal renal function. The water load caused a rise in fetal blood pressure and a fall in plasma osmolality. Since there was no significant increase in free water clearance and fetal plasma osmolality decreased then rose towards control levels, it is concluded that the oral water load was absorbed from the fetal gastrointestinal tract and diffused out of the fetal compartment across the placenta. These experiments show that fetal drinking is probably not responsible for the variability often seen in fetal urine flow and sodium excretion rate.     

Formic Acid Corrosion for the Demonstration of Pulmonary Elastic Tissue

By a revised technique, human pulmonary elastic tissue can be isolated in a form suitable for examination under the stereoscopic microscope. Fresh human lungs from autopsy are fixed by intrabronchial infusion with 10% formalin for 24 hr. Slabs 1.5 cm thick are cut and the formalin removed in running water. One such slab is embedded under intermittent vacuum in an aqueous mixture containing 15% gelatin, 10% glycerol, and 1% phenol; then allowed to gel. Frozen sections 2 mm thick are cut on a large-section MSE sledge microtome. Squares 3 × 3 cm from such a section are corroded for 4-5 days in 88% formic acid at 45 C, washed once with distilled water, and mounted in glychrogel containing 6% gelatin. The elastic tissue network of the lung will have been freed from surrounding elements. The preparation should be stored in a refrigerator. Blocks for thin sections and large thick un-corroded sections can be prepared from the same lung as part of an over-all procedure.