ホーム • Knowledge Pathway • トレーニング教材 • Introduction to Microtomy: Preparing & Sectioning Paraffin Embedded Tissue RELATED CONTENT Knife Angle in Microtomy Techniques to Minimize Articular Cartilage Folding When to use a Vibrating Microtome for Tissue Sectioning Reducing Batch Size to Improve Slide Turnaround Time Introduction to Microtomy: Preparing & Sectioning Paraffin Embedded Tissue Geoffrey Rolls BAppSc, FAIMS Microtomy and Paraffin Section Preparation Creating great paraffin sections using a rotary microtome takes a great deal of skill and experience. "Microtomy and Paraffin Section Preparation" is a great training aid for new microtomists and an excellent refresher for experienced operators. All of the essential aspects of cutting paraffin sections are covered, including: Safety Microtome setup Microtome blades Trimming, facing and roughing blocks Techniques for consistent paraffin sections Microtome maintenance Common microtomy faults Download Microtomy and Paraffin Section Preparation now! Steps to Better Microtomy + Flotation + Section Drying From patient to pathologist, preparing tissue specimens for histological examination requires care, skill and sound procedures. This guide provides practical advice on best practice techniques and simple ways to avoid common errors. Tips for better microtomy + flotation + section drying are highlighted in this guide. We hope each step provides a valuable reminder of good histology practice and helps with troubleshooting when unacceptable results do occur. Want to see all 101 Steps to Better Histology? Download 101 Steps to Better Histology now! Use High Quality Blades High quality, sharp blades are always used for cutting. Blades are used for as long as possible, a few “train lines” are considered acceptable. Image A. A section of spleen (H&E) showing many fine lines due to a defective blade. Image B. Skin sections undergoing flotation. A severe knife line can be seen running right through the tissue. Defects such as this can be easily seen during flotation. Optimize Knife Tilt Angle Knife tilt angle is always optimized for each microtome and blade type. Knife tilt angle is never adjusted when conditions are changed (different microtome, new blade type, different wax etc.). Image This short ribbon of sections that was cut from a cold block shows considerable compression (30–40%). In this case resetting the knife tilt angle overcame the problem. Carefully Trim Blocks Blocks are carefully trimmed to expose tissue. The last few sections are always cut at what will be the final thickness to polish the block face. Blocks are roughly trimmed to save time. The surface is not polished before taking final sections. This often produces a “moth-eaten” appearance in the final section, which is full of small, ragged holes. Image Initial exposure of the tissue (roughing) in this block has pulled fragments from the block surface which has resulted in numerous holes in the final section (H&E). Avoid Freezing Damage Blocks are chilled on a cold wet surface and are always cold when cut (the surface of melting ice is excellent). Blocks are frozen before cutting. This sometimes causes the blocks to crack. Image This block face has cracked because it was frozen to 15°C in a freezer prior to cutting. The cracks may make sectioning and flotation difficult because the wax is no longer bound to the tissue. Use Cold Blocks Blocks are always cold when cut. There is sometimes a delay before final sections are cut from a block. The block may be warm, and this may result in excessive compression of sections. Image A. The distortion of the glomeruli in this kidney section is due to excessive compression when the section was cut (H&E). Image B. Sections from the same block undergoing flotation. The sections on the left were cut without chilling the block while those on the right were cut when the block was cold. Cut Sections Slowly The final sections from each block are cut gently with a uniform, slow rotation. Sections are cut as quickly as possible with a rapid rotation, in the belief that “any section compression will be overcome on the flotation bath.” Image A. Rodent liver (reticulin stain) showing fine chatter due to cutting a cold block of brittle tissue too fast. In this case the problem was overcome by allowing the block to warm slightly then cutting very slowly. Chatter can also result if the paraffin block or blade is poorly secured in the microtome. Image B. This H&E stained section of mucosal tissue shows fine chatter due to cutting a very cold block very quickly. Use Clean Water The water in the flotation bath is replaced regularly. The water in the flotation bath is topped off regularly but replaced only occasionally. Any contaminants in the bath may end upon the slide under the section (fungi, molds, etc.). Image Section from serosa of gastrointestinal tract (H&E). Clusters of weakly staining microorganisms are present within the tissue but could also be seen on the slide, outside the section. The likely source of these contaminating organisms was the flotation bath. Ensure Slides are Clean The cleanliness of slides is always checked before they are used. Handling of slides is kept to a minimum to avoid contamination with squamous cells prior to flotation. Slides are not checked for cleanliness: “As long as the sections stay on the slide during staining, we consider them to be satisfactory.” Dust, organisms and other contaminants can spoil an otherwise good slide. Image A. This section of kidney is spoiled by a black contaminant that was present on the slide prior to use. The deposit could be seen under the section in other parts of the slide. Image B. A section of lung containing stained adhesive “pools” which have been formed as the section dried. The adhesive (probably gelatin based) was present in the flotation bath. The protein content of the adhesive has been concentrated as the water evaporated. Proper draining of the section prior to drying may have avoided the problem. Avoid Cross-contamination The water surface is always skimmed between specimens to avoid contamination of one section with cells from another. The water surface is not skimmed between every block. This can result in specimen-to-specimen contamination which can cause confusion and even an inaccurate diagnosis. Image A section of cardiac muscle has been contaminated with a fragment of thyroid from another case. This example of specimen-to-specimen transfer occurred on the flotation bath. Avoid Contamination with Squames Care is taken not to brush hair or hands while floating-out sections (squames can contaminate sections). “Some of our staff produce slides containing many squames. They seem unaware that this can be avoided.” Image A kidney section containing many extraneous squames that were deposited on the surface of the section while it was on the flotation bath. They adhere firmly and are subsequently stained with eosin. Don’t Float from Multiple Blocks Sections from more than one block (case) are never simultaneously floated on the water bath. Sometimes sections from two or more blocks (cases) are left floating-out simultaneously. This is a dangerous practice that can lead to inaccurate identification of specimens. There is a particular risk when the sections happen to be from the same type of specimen. Image Here sections from two different cases are being floated-out simultaneously. This practice can result in confusion and lead to inaccurate identification of sections. Check Water Temperature Flotation bath temperature is carefully checked. A temperature 4–5°C below the melting point of the wax is optimal. Sections should readily flatten but the wax should not melt. If sections are left on the flotation bath for more than 15 seconds, the wax melts. Although this may seem to make the process faster, it can rapidly cause over-expansion and tissue and cell damage. Image These sections of skin clearly show cracks and excessive separation of layers, the typical effects of over-expansion. Poorly processed tissue is very prone to this problem. Avoid Wrinkles in Sections Sections flatten readily on the flotation bath. Sections never quite flatten on the flotation bath. The bath may be too cold, and the sections may remain wrinkled when picked up on the slide. Image In this case, flotation has not overcome the wrinkles produced during the cutting of these sections. Better cutting technique and slightly warmer water would overcome this problem. Avoid Over-expanding Sections Sections are left on the flotation bath for just long enough to flatten then promptly picked up on a slide. For convenience, some sections are left for extended periods on the flotation bath. This can cause over-expansion and tissue damage (particularly to delicate specimens such as lymphoid tissue). Image A. This section of intestinal mucosa stained with PAS shows a lamina propria that is over-expanded (shows excessive separation from the intestinal glands). In this case, the section was floated for too long on a bath that was too hot. Image B. A section of lymphoid tissue that has cracked due to over-expansion on the flotation bath. Lymphoid and hematopoietic tissues are particularly prone to damage in this way. Don’t Damage Floating Sections Extreme care is taken to avoid damaging floating sections when mechanically removing wrinkles with a brush or forceps. Wrinkles are vigorously removed from floating sections with a brush or forceps. Macroscopic and microscopic damage can easily be caused by this procedure. Image A section of cardiac muscle shows mechanical damage (gouging), caused when attempting to remove a fold in the section (heart, H&E). Carefully Choose Sections The first one or two sections in a ribbon are never picked up on slides. The first and second sections in a ribbon are selected for mounting because they look better than the later sections. They look better because they are invariably thicker due to the expansion of the cold block during the first couple of passes across the knife. Image The sections in the ribbon prepared from this block are numbered in the order in which they were cut. Note that the first couple of sections are widest (least compressed) but as the block warmed the sections got narrower (more compressed). Although the microtome was set on 3 µm the first couple of sections would be 4–5 µm thick due to thermal expansion. Prevent Bubbles Under Sections Care is taken to avoid the formation of air bubbles in the flotation bath. Any visible bubbles are dislodged before the sections are laid on the water. Small air bubbles in the flotation bath are ignored. Any bubbles that are trapped under the section seem to disappear as the section dries. Although the bubbles may seem to disappear, the areas in the section above the bubble are often distorted and are likely to float off during staining. Image A liver section stained H&E, showing a circular, cracked area where the section has lifted. The cause was a bubble that lodged under the section during flotation and prevented proper flattening and adhesion. Prevent Section Lifting The use of “sticky” (charged) slides or section adhesives such as AAS is considered and used appropriately. Sometimes sections float off during staining (particularly during antigen retrieval for IHC or when methods require the use of heat). Charged slides or section adhesives are required in these circumstances. Image This slide shows an area where the section has lifted and been deposited on adjacent tissue (lung, H&E). Drain Before Drying Sections are drained briefly before being placed in the slide dryer or onto a hotplate. Sections are not drained properly before being dried horizontally. Sections move on the slide and sometimes do not dry flat. Image A. This section was dried horizontally without effective preliminary draining. As a result, a raised out-of-focus area is visible in the center of the field. Image B. This section has just been picked up from the flotation bath and will be drained vertically for a brief time before being placed in the slide dryer. This will avoid the problem shown in A. Monitor Drying Temperature The temperature of the slide dryer is carefully monitored. Sometimes the slide dryer is very hot. Excessive heat can produce hot spots in sections and cause uneven staining. Image This section of prostate shows the features of “nuclear meltdown”, one possible cause being excessive heat when drying slides. Faulty tissue processing can produce a similar effect. Nuclear meltdown is typically seen at the perimeter of specimens and usually affects epithelial tissue. Nuclei show uneven staining, sometimes appearing pink or very blue and completely lacking detail. Dry for Appropriate Time The minimum and maximum slide drying time is monitored. Slide drying times vary considerably. Extended drying at higher temperatures may be detrimental to sections. Image Dieser Lymphknotenschnitt wurde zu lange und bei zu hoher Temperatur getrocknet und weist zahlreiche Risse auf. Solche Risse können auch durch andere Fehler in der Präparaterstellung verursacht werden, u. a. durch eine Überinfiltration. H&E-Färbung. Download 101 Steps to Better Histology now! About the presenter Geoffrey Rolls , BAppSc, FAIMS Geoffrey Rolls is a Histology Consultant with decades of experience in the field. He is a former Senior Lecturer in histopathology in the Department of Laboratory Medicine, RMIT University in Melbourne, Australia. Related Content Knife Angle in Microtomy Techniques to Minimize Articular Cartilage Folding When to use a Vibrating Microtome for Tissue Sectioning Reducing Batch Size to Improve Slide Turnaround Time Leica Biosystems Knowledge Pathway content is subject to the Leica Biosystems website terms of use, available at: Legal Notice. The content, including webinars, training presentations and related materials is intended to provide general information regarding particular subjects of interest to health care professionals and is not intended to be, and should not be construed as, medical, regulatory or legal advice. 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