SU1773409A1 - Method for assessment of non-specific reactivity in sheep - Google Patents

Description

(54) MEANS FOR DETERMINING THE NON-SPECIFIC REACTIVITY OF SHEEP (57) Usage: experimental and veterinary immunology. Essence! determination of nonspecific reactivity of sheep using hemolysin, which is used at a dilution of 1: 8-1: 16. Hemolysin is mixed with the peripheral blood of the test animal, incubated for 18 hours at 20-24 ° C in capillaries and the results of the reaction according to the erythrocyte sedimentation rate and the degree of hemolysis in the experimental and control samples are taken into account. According to the results of the reaction, the index of nonspecific reactivity of animals is determined. 3 tab.

The invention relates to immunology and can be used to determine the physiological state of the body.

Hemolysin, an inactivated blood serum of a rabbit immunized with sheep erythrocytes, is known as a drug that is widely used in laboratory practice as a diagnosticum. Specific hemolytic serum, which lyses sheep erythrocytes in a high titer, is used in the complement binding reaction (Handbook of microbiological and virological research methods. / Ed. By MO Birger. - M .: Medicine. 1982, p. 464).

It is also known to use hemolysin in complement titration. Its activity is determined in the same hemolytic system that is used for the complement binding reaction (standard sheep erythrocytes and antiserum). The complement content is judged by the smallest amount of the studied serum, which contributes to the complete or 50% hemolysis of sensitized erythrocytes [1].

There is a known method for determining the immunological reactivity of individuals, including incubating blood samples with a testing biological fluid, and a species-specific antiserum is used as a testing biological fluid, which is mixed with the peripheral blood of the subject in a ratio of 1: 2, incubated for 18 hours at 20-24 ° C in capillaries, and the results of re- | shares are taken into account according to the erythrocyte sedimentation rate and the degree of cytolysis in the experimental and control samples.

The disadvantage of this method is that. that for its implementation in a laboratory, it is necessary to prepare a species-specific serum, which is associated with

1773409 A1 great difficulties (the presence of laboratory animals, cost and time). In addition, sera obtained in different laboratories and at different times are not stable. The quality of the obtained antisera depends on many factors associated with the technology of their production, including: the degree of antigen purification, the level of the immune response of laboratory animals, and others.

The aim of the invention is to expand the arsenal of tools for determining the nonspecific reactivity of the organism and to increase the possibility of their practical application.

This goal is achieved by the use of hemolysin as a tool for the determination of non-specific reactivity in sheep. Determination of the reactivity of the sheep population is carried out in vitro by mixing hemolytic serum with the peripheral blood of the test animal, incubating the mixture in capillaries, followed by taking into account the results of the reaction after 18 hours according to the degree of cytolysis in the experimental and control samples.

The essence of the technical solution is as follows.

Hemolytic serum ratio. 1: 2 is mixed with the peripheral blood of the test animal, incubated for 18 hours at 20-24 ° C in capillaries, and the reaction results are taken into account according to the erythrocyte sedimentation rate and the degree of hemolysis in the experimental and control samples.

Species-specific antibodies of hemolytic serum, under the influence of the complement of the studied animal, react with erythrocyte antigens, which leads to their agglutination and hemolysis. The cytotoxic effect of hemolysin depends on the complement content in the blood of the studied animal, as well as on the functional activity of blood cells and the genotypic characteristics of the organism.

The proposed tool has been tested on ewes, newborn lambs and is illustrated by examples.

PRI me R 1. Prepared various dilutions of hemolysin in saline and set the drop hemagglutination reaction with the blood of the animal under study. Hemolytic serum for the complement fixation reaction was used in a dilution of 1/8, 1/16, 1/32, 1/64, 1/128.

One drop of the blood of the test animal was applied to a glass slide, then one drop of hemolysin was added, quickly stirred with a glass rod, and after 3-5 min the results of the reaction in crosses were taken into account.

As can be seen from the data presented in table. 1, the highest dilution of hemolysin, with which agglutination of erythrocytes in the blood samples under study is observed, was 1/128. However, in some animals (No. 35; 9586; 4570, etc.) the reaction was negative. The most pronounced reaction, with an intensity of at least two crosses, was noted in a dilution of hemolytic serum equal to 1/16. In this regard, hemolytic serum 1:16 was taken to determine the immunological reactivity of animals.

PRI me R 2. Hemolysin was taken into a capillary pipette of the Panchenkov apparatus of 1/2 volume of 50 mm and poured into a well of a glass slide. Then blood (1.00 mm) was taken with the same pipette and also poured into the well. The blood of the test animal was thoroughly mixed with the antiserum, and the resulting mixture was drawn into a pipette and placed in a rack. Due to the fact that hemolysin was mixed with the blood of the studied animal at a 1: 2 dilution, its working dilution was 1: 8.

A control sample was also set for each animal separately. In the control capillary, physiological saline was used instead of hemolytic serum.

Accounting for the reaction (control and experiment) was carried out after 18 hours according to the erythrocyte sedimentation rate (the height of the column of settled erythrocytes), as well as the degree of cytolysis.

The index of nonspecific reactivity was determined by the formula

INR = (AB): A + (C-D): C, where PNR is the index of nonspecific reactivity;

Ά - the height of the column of settled erythrocytes in the experimental capillary;

B - the height of the column of settled erythrocytes in the control capillary;

C - the degree of hemolysis in crosses in the test capillary;

D - degree of hemolysis in crosses in the control capillary.

The results of accounting for the reaction for individual animals are presented in table. 2.

As can be seen from the data presented in table. 2, the height of the column of settled erythrocytes in the experimental and control capillaries in animals was different. The most significant difference was noted in animal no. 4027 (7 mm in the control and 67 mm in the experiment), which corresponded to the highest reactivity index. In animal no. 10C4, the difference was less significant; 1 mm, and the index of nonspecific reactivity was 0.07.

Example 3. According to the described methodology, the nonspecific reactivity of 92 ewes and 97 lambs born by them was assessed. As a result of studies (Table 3), it was found that the average values of the index of nonspecific reactivity in ewes were significantly higher than in lambs.

As you can see, the differences between groups of animals, not only in average values, but also in the nature of the distribution of values are statistically significant. The variance of the reactivity index in lambs was more pronounced than in queens. The coefficient of variation of the index of nonspecific reactivity in lambs was 98.6%, and in queens 65.1%.

When comparing the results of the reaction in ewes and lambs born from them, it was found that in lambs there were no cases of hemolysis of erythrocytes with the addition of hemolytic serum. On the contrary, in ewes, such cases were recorded more often. Apparently this should be explained by the lack of complement in the blood of newborn lambs.

Since the complement system plays an important role in maintaining homeostasis, the indicators of this reaction reflect the characteristics of the body's reactivity.

Thus, the proposed tool, when used to determine nonspecific reactivity, can significantly expand the possibilities of practical application, especially in a mass survey of livestock.

The use of a known diagnosticum as a means for determining nonspecific reactivity has the advantage of being produced by the biological industry, standardized and available in any district laboratory.

Since hemolytic serum exhibits its effect in the presence of complement, the manifestation of agglutination and hemolysis caused by the action of antibodies depends on the reactivity of the complement contained in the blood of the animal under study. On the other hand, the results of the reaction also depend on the specificity of antigens adsorbed on the surface of erythrocytes.

Claims (19)

30 Image f o rmule The use of hemolysin as a means for determining the nonspecific reactivity of sheep. Table 1 But- measures Inventory number of the animal The results of the reaction depending on the dilution of hemolysin in a saline medium 1/8 1/16 1/32 1/64 1/128 1 09661 + -H- + ++ 4- + -n-b -H- 4- 2 B / 35 ++++ ++++ + 4- + - 3 1294 4-4-H- + -H- + 4-H- ++ 4- 4 04033 4- + 4-4- 4-4-4-4- +++ ++ + 5 9586 +4 - + - I- ++++ ++ - - 6 2177 -H-H- -H - ++ 4-4-4- 4-4- 4- 7 4570 4- + 4- + -I - ++ 4- 4-4- - - eight 07941 +++ 4-4- - - - nine 02966 ++++ 4-4-H- -H - ++ ++ - ten 2464 ++++ + -H- + 4-4- - - eleven 4815 4 - +++ ++++ ++ - - 12 2257 + 4-H -I - ++ -1-I-4- 4-4- -n- 13 07276 + - (+ 4- ++++ 4-4- - - fourteen 4593 +++ 4-4-4- + - - 15 07050 ++++ 4-4- 4-4-4- 4- - 16 1520 ++++ I -f-f-f- + 4 '+ + - 17 1644 4- ₊ 4_ ₊ 4 -4 -4- 4- - eighteen 0706 +++ 4-4-4- 4- - - 19 1971 ++ - H- 4-4-4-4- 4-H- + 4- [twenty 9981 +4 - ++ 4-4-4-4- 4-H- 4- - table 2 Number Inventory number of the animal Column height of settled erythrocytes, mm Immunological reactivity index control AN EXPERIENCE 12 3 4 5 6 7 eight nine ten eleven 12 13 fourteen 15 16 17 1313 1004 4027 1177 4093 1535 7718 4502 4291 2514 2903 1799 9115 7340 4893 9645 7108 7 fourteen 7 5 ten 13 7 10 13 eleven 15 5 15 21 eight eighteen 5 ten 15 67 thirty 55 19 19 15 16 49 70 17 thirty 40 16 55 twenty 0.30 0.07 0.89 0.83 0.82 0.32 0.63 0.33 0.19 0.78 0.79 0.71 0.50 0.47 0.50 0.67 0.75 Table 3 Group of animals Number of animals Nonspecific reactivity index mean values M + frequency distribution,% less than the M value in the group more than M Uterus 92 0.46 ± 0.03 38.90 61.10 Lambs 97 0.22 ± 0.02 61.50 38.50 Difference criterion td = 6.70 L = 1:54 Credibility P <0.001 P <0.05 Compiled by A. Dmitriev