David H. Lloyd

Practical Equine Dermatology


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       History of skin problems in related animals.

       Type of husbandry and use:Length of time owned.Use – competitions, general riding, breeding, racing.Feeding regimen.Periods spent in stable or at pasture.Type of stable and bedding – stable hygiene, contamination.Conditions in paddocks – mature meadow pasture or new grass ley, proximity of water, trees.Seasonal changes in management.Routine health care procedures – vaccination, deworming.Figure 1.1 Taking the history. Components and the sequence of the history taking process. Analysis of the history should enable the clinician to construct an initial list of differential diagnoses that may help to focus the clinical examination along particular diagnostic lines. It may enable the diagnostic process to be abbreviated where a likely diagnosis is indicated, or it may point towards the need for a more detailed approach.Grooming procedures – sharing of grooming kit, tack, grooms.Equipment used in contact with horse – boots, bandages, saddle cloths, rugs.Contact with other horses, other species – opportunities for disease transmission.History of the current problem.First signs, progression, response to treatment and management changes.Seasonal effects.Previous episodes of disease.Results of any diagnostic tests.Current or recent therapy – includes questions about use of over‐the‐counter and non‐veterinary products.Evidence of transmission – lesions in other horses, other species, humans.General health – concurrent or previous conditions.

      A full clinical examination to assess both the general health status and the skin is necessary in most cases. Ensure that the animal is adequately restrained and that you have sufficient light. Work systematically down each body region, beginning at the head and ending at the tail and perineal region. Be sure to include all aspects of the feet including the coronary band and the frog. The skin may need to be cleaned to observe some lesions. In some instances, sedation may be necessary.

      It may be helpful to visit and examine the paddocks and exercise areas used.

Schematic illustration of example of an examination form for recording distribution and nature of lesions in equine dermatology cases.

      The history and clinical examination should enable you to formulate a list of differential diagnoses. It may help to create a problem list, identifying the relevant historical features and predominant clinical signs, categorising them as contagious or non‐contagious, and allocating the disease within the following groups, which form the basis for the problem‐orientated approach in this book:

       Pruritic

       Crusting and scaling

       Ulcerative and erosive

       Nodular or swollen

       Alopecia/hair coat changes

       Pigmentary disorders

      A diagnostic plan can then be constructed, diagnostic procedures selected, and samples collected. Sample collection may include the following techniques.

       Hair plucks

      Useful to determine whether the lesions of alopecia or hypotrichosis are due to self‐inflicted damage (fractured hair shafts, split ends) indicating that the condition is pruritic, or due to abnormal hair growth (absence of anagen roots, abnormal catagen roots), and to examine for dermatophytes and for parasite eggs.

       Choose fresh, unmedicated lesions.

       For suspected dermatophytosis, where cultures are required, first lightly clean the areas to be sampled with 70% alcohol (to reduce contaminant organisms).

       Tissue or epilation forceps can be used to grasp gently and pull out hairs from the periphery of the lesion.

       Samples for microscopy can be placed on adhesive tape wrapped around a microscope slide and mounted in a drop of liquid paraffin just prior to examination.

       Samples for fungal culture submission should be held in paper or sterile, non‐airtight containers to prevent a humid environment that might support the growth of saprophytic organisms.

       Crusts

      Useful for cytological examination looking for bacterial organisms (particularly Dermatophilus) and for submission for fungal and bacterial culture.

       Choose a fresh, unmedicated lesion.

       Impression smears of the underside of freshly removed crusts, stained with a rapid Romanowsky‐type stain (e.g. Diff‐Quik, Hemacolor, Rapi‐Diff, Speedy‐Diff) or Gram’s stain, can provide a quick method of diagnosis for dermatophilosis.

       Crusts can be collected and held in paper envelopes or sterile containers for transport to the laboratory.

       Dried crusts can be emulsified in a drop of sterile saline on a slide, warmed to allow rehydration of material, prior to air‐drying and fixing (heat fixation for Gram’s stain, methanol/ethanol fixation for rapid‐differentiating Romanowsky‐type stains) for cytological examination and identification of bacterial and fungal organisms.

       Coat brushings

      These allow for examination for surface‐living external parasites and dermatophytes where the lesions are diffuse or extensive. Scrapings are better for deeper resident mite infestations.

       Use a sterile scalp brush or new toothbrush to brush firmly over the lesions (Mackenzie brush technique; Figures 1.4a and b). Place the brush in a paper envelope to protect it prior to submission for dermatophyte culture.

       A scalp brush or wooden tongue depressor can be used to collect debris directly into a sterile Petri dish for external parasites. Material should be examined promptly as chorioptic mange mites are highly motile and easily lost from sample containers.

Photos depict (a) a coarse-toothed brush facilitates sampling of large areas of skin and coat. (b) Here Microsporum canis has been isolated using this technique.