Tissue Cutting Preparation for Histological Examination
An essential point in preparing tissues for section is to get them as fresh as possible. So that anything in the nature of retrogressive changes in the cells may be absolutely avoided tissue cutting. On this account other animals are, for the most part, used instead of man. As there is always more or less delay in obtaining anything from the post mortem room. The examination of the corpse for histological examination being not usually made till many hours after death. Neither can the organs be relied upon as being healthy.
The usual method of procedure when organs, such as the liver or kidneys of a small mammal, as the cat or rabbit, arc required to be hardened, may be shortly described as follows.
Step 1 – Dead body
The animal is first killed, usually by placing it under a bell jar. This jar is just large enough to accommodate it. Therefore, with a piece of tow soaked in chloroform or ether. When dead it is removed, and body is washed including the abdomen thoroughly moistened with a wet sponge before making an incision.
Step 2 – Losing the skin for tissue cutting
In order to avoid the inconvenience arising from the loose fur if the skin is cut without this pre caution being taken. The abdominal wall may now be cut with blunt pointed scissors in the middle line from the sternum to just above the pubes. And again transversely about the level of the umbilicus.
Step 3 – Cutting opening the body cavity
The contents of the cavity are next exposed by holding back the flaps. The liver and kidneys are removed. These must then be moved rapidly to and from in a basin of water, to remove the superfluous blood. Water not being an indifferent fluid quickly affects the tissues. So that this rough process of cleansing is made as short as possible. But in all cases where the tissue cutting is such that contact with ordinary water will be injurious, normal saline should be used instead.
Step 4 – Separating the body organs
The organs are now cut with a sharp scalpel or razor into suitable pieces. In ordinary cases should be less than half an inch in their narrowest diameter. The smaller the pieces can be made consistently with the sections subsequently derived from them demonstrating the structure of the organ. The better as the penetration of the hardening reagent is the more rapid. It is sometimes convenient to cut the pieces rather large at first, re-cutting them more carefully the following day.
Step 5 – Washing, Tissue cutting and organ preserving
Rapidly wash the pieces as soon as cut in water or normal saline, to again remove the blood. Place them in the fluid in which they are to be hardened. Of these fluids there is a considerable choice. It depends greatly on what the organ is, as to which is selected. Some hardening reagents, however, may almost be termed general ones. That is to say, they are applicable to the treatment of nearly all tissues.
Whereas others, on the other hand, are only used for special purposes. Whichever reagent is used, there are certain rules to be attended to in the process of hardening, which hold good for all. It is of primary importance that there should be an abundance of the fluid used. It should be largely in excess of the pieces of tissue placed in it, for if only sufficient to cover them in the vessel in which they are placed. It very soon loses its strength, and if not quickly replaced by fresh fluid, changes in the tissue rapidly supervene.
Step 6 – Preserving the tissue for future tissue cutting
On the second day the fluid, which will have become more or less turbid, should be poured off. The bottle containing the tissues rinsed out with water, and a fresh supply of the reagent added. It will be noted we are now speaking of the commoner reagents, such as MUiler’s fluid, MUiier and spirit, etc. After the second day, this should bechanged as often as it becomes turbid. How often this occurs will depend largely upon the relative quantity of the fluid and the tissue. The greater the proportion of the former the less frequently will it require to be changed. Also on the nature of the tissue dealt with. Pieces of the lung require the fluid to be comparatively seldom changed. Those of the liver more frequently. Roughly speaking, every third or fourth day would suffice in most cases.
Step 7 – Harding of cut tissues
Though as the hardening progressed, once in five, six, or more days, would be sufficient. The process usually occupies from three to five weeks, though in some cases a shorter time suffices. After hardening, the tissues are pre served in methylated spirit for future tissue cutting.
Step 8 – Tissue Cutting
Various methods are adopted to ensure every piece being thoroughly exposed to the action of the reagent. To this end a layer of tow or cotton wool may be placed at the bottom of the vessel for them to rest upon. Sometimes it is convenient to suspend them separately by means of thread, the ends of the threads being attached to a glass rod crossing the mouth of the vessel. Or they may be fixed in any other convenient way. As a general rule this is unnecessary if there is plenty of fluid, and too many pieces are not placed in the same vessel.