IMPACT OF THE DRUG REOMANNISOL IN THE MODEL OF AN EXPERIMENTAL DIABETIC FOOT

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ABSTRACT

The aim of the study was to learn of the effect of the new drug "Reomannisol" on wound healing, taking into account

pathomorphological aspects in the complex treatment of experimental diabetic foot syndrome.

Material and methods.

An experimental study was carried out on 140 outbred male rats weighing 220-250 g, kept in

the TMA vivarium. The experimental animals were divided into 4 groups: the 1st group was intact; 2nd group

–

the

creation of an experimental model of alloxan diabetes mellitus; 3rd control group - against the background of alloxan

diabetes, the creation of an experimental model of a diabetic foot using traditional complex treatment; 4th

experimental group - on an experimental model of diabetic foot - traditional treatment and reomannisol. On the skin

of each rat’s right hind paw’s footpad, a full

-thickness rectangular wound measuring 2 mm×5 mm was created with a

scalpel. Every day, the wounds were treated with the traditional method of treatment (5% alcohol solution of iodine

and levomekol ointment) until the end of the experiment, for the experimental group, the local traditional method of

treatment and intraperitoneal administration of the new Reomannisol preparation were used 1 time per day at a dose

of 1 ml of Reomannisol per 100 g of animal div weight for 5 days.

Results.

By the 10th day in the experimental group, an independent almost complete closure of the wound defect and

hair growth around the wound was noted. In the control group, on the 10th day, a wound defect of about 4.9 ± 0.05

mm2 remained, the wound healed on the 14th day of the experiment.

Research Article

IMPACT OF THE DRUG REOMANNISOL IN THE MODEL OF AN
EXPERIMENTAL DIABETIC FOOT

Submission Date:

November 12, 2023,

Accepted Date:

November 17, 2023,

Published Date:

November 22, 2023

Crossref doi:

https://doi.org/10.37547/ijmscr/Volume03Issue11-08

Ernazarov Khojimurod Irsaliyevich

Phd, General Surgery Department No.2, Tashkent Medical Academy, Uzbekistan

Journal

Website:

https://theusajournals.
com/index.php/ijmscr

Copyright:

Original

content from this work
may be used under the
terms of the creative
commons

attributes

4.0 licence.

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Conclusion:

The use of local treatment and reomannisol can enhance angiogenesis in the early stages of the

experiment and restore disturbed microcirculation, increase macrophage response, fibroblast proliferation,

maturation and remodeling of granulation tissue and its epithelization, reduce the inflammatory reaction, which leads

to more effective and early healing of the wound area.

KEYWORDS

Experimental model of diabetic foot, experimental animals, diabetes mellitus, alloxan, surgical debridement,

reomannisol.

INTRODUCTION

Currently, one of the leading places in terms of growth

rates of morbidity, disability, and mortality was

occupied by diabetes mellitus (DM) among the so-

called "diseases of civilization" [3]. Today, over 460

million people are suffering globally from diabetes;

according to the predicted facts announced by the

International Diabetes Federation, by 2040 the number

of patients will increase up to 642 million [11].

Diabetes mellitus is accompanied by the development

of complications, including diabetic foot syndrome

(DFS), one of the leading clinical symptoms of which is

the persistence of an ulcer on the skin of the lower

extremities [14].

Delayed wound healing is one of the complications of

the disease due to multiple factors including poor

circulation [13], prolonged inflammation, and

hyperglycemia. It is a common cause of morbidity and

mortality in patients with DM [18]. When the wound

becomes chronic, it is prone to developing foot ulcers,

including neuropathy and foot deformities [13]. Foot

ulcers in DM are the cause of more than 50% of all non-

traumatic leg amputations [22]. Evidence has shown

that hyperglycemia is one of the main factors

contributing to slow wound healing [18] by increasing

cell apoptosis and decreasing cell survival in diabetic

wounds. It has been shown to inhibit endothelial cell

and fibroblast proliferation in humans [23], up to 75%

slower in adult mice with DM compared to control mice

[19].

At the present stage in experimental diabetology, the

most widespread chemical model of diabetes mellitus

uses substances that destroy β

-cells of the islets of

Langerhans [12, 15]. This study describes a model of

diabetes mellitus in rats, induced by the introduction of

a reduced dose of alloxan, which significantly reduces

the number of animal deaths.

The alloxan model of diabetes mellitus is one of the

most widespread and studied. It is actively used by

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researchers around the world. Alloxan is a structural

analog of glucose, due to which it accumulates in

pancreatic β

-cells and leads to their death, followed by

the development of diabetes. At the same time,

damage to β

-cells is accompanied by degenerative

changes in the kidneys and liver, which leads to high

mortality in laboratory animals on the first day after

alloxan administration. The problem of violations of

several types of metabolism with the introduction of

alloxan, the prevalence of manifestations of oxidative

stress as a typical pathological process in case of

damage to the key organ involved in all types of

metabolic processes (liver) dictate the need to

prescribe pathogenetic drugs from the group of

metabolic correctors with hepatoprotective and

antioxidant orientation. One of the promising new

drugs in this area is Rheomannisol (LLC "REKA-MED

FARM" Republic of Uzbekistan) - a complex drug with

antihypoxic, antioxidant, rheological, anti-shock,

detoxifying,

diuretic

action.

The

main

pharmacologically active substances are sodium

succinate and mannitol.

Aim of the study. Study of the effect of the new drug

"Rheomannisol" on endogenous intoxication and

wound healing, taking morphological aspects into the

complex treatment of experimental diabetic foot

syndrome.

Materials and research methods. The work was done

on experimental material. Healthy rats were selected

for the experiment. Experimental studies were carried

out on 140 outbred male rats weighing 220-250 g, kept

in the Tashkent Medical Academy (TMA) vivarium. The

rats were kept under optimal conditions, all rats lived

in a room with a 12-hour light-dark cycle and a constant

temperature of 22-25°C, with free access to water. All

rats were given a sufficient amount of a normal rodent

diet ad libitum. (diet for rodents, State standard No.

GOST R50258

–

92) and tap water daily. Operations and

all manipulations with animals were carried out using

general anesthesia, in compliance with the principles

of humanity outlined in the directives of the European

Community (86/609/EEC) and the Declaration of

Helsinki, by the "Rules for working with experimental

animals". The experimental animals were divided into

4 groups: the 1st group was intact; 2nd group

–

the

creation of an experimental model of alloxan diabetes

mellitus; 3rd control group - against the background of

alloxan diabetes, the creation of an experimental

model of a diabetic foot using traditional complex

treatment; 4th experimental group - on an

experimental model of diabetic foot - traditional

treatment and reomannisol.

After a 24-hour fast, the rats were weighed. A 2%

solution of alloxan diluted in 0.9% saline was

administered intraperitoneally as a single dose,

corresponding to a dose of 20, 15, 12 mg of alloxan per

100 g of animal weight. Food and water were given to

animals only 30 minutes after drug administration. On

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the 3rd day, the level of glucose in the blood was

assessed.

Determination of glucose concentration in the

peripheral blood of animals. Diabetes was confirmed 3

days after the blood glucose concentration was

determined. Peripheral blood glucose concentration

was measured with an “Accu Chek Active” glucometer

(Roche

Diagnostics,

Germany),

the

linear

measurement range was 0.6

–

33.3 mmol/L. Blood

sampling to study the level of glycemia was performed

from an incision in the tip of the tail. An experimental

model of diabetes mellitus (type I diabetes) has been

obtained. The day of verification of diabetes mellitus

was considered the zero-day of its development.

Surgical procedure. On the day of verification, the skin

surface of the right footpad was shaved and cleaned

with a 70% ethanol wipe. On the skin of each rat’s right

hind paw’s footpad, a full

-thickness rectangular wound

measuring 2 mm × 5 mm was created with a scalpel

[14]. The scalpel and scissor wounds (Day 0) were of

similar size and shape with minimal or no bleeding in all

groups. Every day, the wounds were treated with the

traditional method of treatment (5% alcohol solution of

iodine and levomekol ointment), until the end of the

experiment, also for the experimental group, in

addition to the local traditional method of treatment,

a new drug Reomannisol (JV LLC REKA-MED FARM,

Republic of Uzbekistan) was used, which was

administered intraperitoneally once a day for 5 days, in

single doses of the therapeutic range for humans,

taking into account differences in relative div surface

area [1]. In all cases, the average dose of the studied

range was 1 ml of Reomannisol per 100 g of the

calculated equivalent mean therapeutic dose (EMTD).

The development of the disease was assessed by the

condition of the animals, lethality was recorded in

groups, and recorded according to clinical symptoms

(polyuria, polydipsia, polyphagia, weight loss, coat)

and blood glucose levels. The wool of animals normally

has a peculiar luster and is usually adjacent to the skin.

The amount of water drunk by the rats was determined

individually by measuring its volume with a measuring

cylinder before and after the animals took water. To

assess the daily values of diuresis, an individual urine

collection was performed using urinals.

Rats were taken out of the experiment by decapitation

on days 1, 3, 7, 10, 14, blood was taken for laboratory

examinations: biochemical analyzes (total protein,

ALT, AST, glucose, creatinine, urea), products of lipid

peroxidation (LPO) (malondialdehyde - MDA),

indicators endogenous intoxication (MWM, SCE),

morphological studies of tissues taken from the wound

zone and the surrounding intact area were carried out.

At each time, sampling for analysis was carried out in

10 animals of each group.

Biochemical analyzes (the activity of aspartate

aminotransferase (AST), alanine aminotransferase

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(ALT), total protein, glucose, creatinine, urea) were

measured on a biochemical analyzer photometer

Mindray BA-88A (Mindray, China), using a set of

chemical

reagents

manufactured

by

Human

(Germany).

Determination of malondialdehyde (MDA) using

thiobarbituric acid. At high temperatures in an acidic

medium, MDA reacts with 2-thiobarbituric acid,

forming a colored trimethylene complex, with an

absorption maximum at 532 nm on an SF-46

spectrophotometer (Russia). The molar coefficient

was used - 1.56x105cm-1 x M-1. The MDA level was

expressed in µmol/L [9].

A biochemical method for determining endogenous

intoxication, which consists in choosing the level of

medium-weight molecules in the blood serum. Medium

weight molecules (MWM) are an integral biochemical

marker of endogenous intoxication (EI). In the blood

plasma of all subjects, the level of MWM was assessed.

For this, a screening method for determining

molecules was used, this method includes taking

blood, separating serum from blood cells by

centrifugation, obtaining a protein-free sample by

adding 0.5 ml of 10% trichloroacetic acid to 1 ml of blood

serum, and centrifuging for 30 minutes at 3000 rpm in

min. Next, 4.5 ml of distilled water is added to 0.5 ml of

the supernatant and the optical density of the sample

is determined on a spectrophotometer with a wave

characteristic of 254 nm. The content of molecules of

average mass is determined by the size of the optical

sample, and the presence of endogenous intoxication

is judged by their high degree. Measurement of the

level of MWM and oligopeptides allows you to

calculate the Integral index of intoxication. To

calculate the optical density in the ultraviolet region of

the spectrum, a UNICO 2800 spectrophotometer

(USA) was used [2].

Determination of the concentration of oligopeptides

(OP). The method for determining the content of OP

according to Lowry (1956) was used. To do this, 1 ml of

a weakly acidic supernatant diluted 10 times with

distilled water was taken, 2 ml of an alkali-copper

reagent was added, and left for 10 min. at room

temperature, then 0.2 ml of the Folin-CiocALTeu

reagent was added, stirred, and after 30-40 minutes.

the optical density was measured at 750 nm in a cell

with a length of 5 mm on a UNICO 2800

spectrophotometer (USA) [20].

The sorption capacity of erythrocytes (SCE) was

determined by a method based on the idea of an

erythrocyte as a universal adsorbent [10]. To do this, 1

ml of erythrocyte suspension was transferred into a

test tube with 3 ml of 0.025% methylene blue in

physiological saline. After a 10-minute incubation at

room temperature, the sample was centrifuged for 10

minutes. at 3,000 rpm the optical density of the

supernatant and the initial solution of methylene blue

was determined concerning physiological saline at a

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wavelength of 630 nm using a UNICO 2800

spectrophotometer (USA). The amount of absorbed

dye was expressed as a percentage [10].

Evaluation of the effectiveness of the drug was carried

out based on, also, a visual examination of the animals

and their wounds. The criteria for the effectiveness of

the drug for the wound were: focusing on the severity

and duration of inflammatory manifestations in the

wound area (edema, hyperemia, wound exudate), the

state of the wound bottom; the appearance of

granulation tissue; reduction in the area of the wound

defect; the appearance of marginal epithelialization;

acceleration of wound healing,

The L.N. Popov test was used to determine the area of

the wound. A sterile cellophane plate is placed on the

wound and the contour of the wound is applied to it.

The drawing is transferred to graph paper and the area

of the wound is calculated.

Where ΔS

is the desired value in cm2;

S is the area of the wound in the previous

measurement in cm2;

Sn - the size of the area of the wound at the moment in

cm2;

t is the number of days between measurements [5].

The research methods described in the classical

manuals on histomorphology were applied in the work

[18]. Pieces from a diabetic foot, pancreas, and liver

were fixed in Carnoy's solution (the composition of the

fixative was glacial acetic acid, 10 parts; chloroform, 30

parts; ethyl alcohol, 60 parts). Fixing the pieces for 2-4

hours, then placing the pieces in 96% alcohol. Carrying

out the wiring in the usual way and pouring in paraffin.

Making histological sections with a thickness of 5-6

microns on a sledge microtome, deparaffinization on a

thermostat, and staining with hematoxylin and eosin.

It is the most common method of staining histological

sections. Paraffin sections are deparaffinized in

chloroform and washed in distilled water, then a

hematoxylin solution is poured onto the sections for 3

minutes. Rinse in tap water for 10 minutes and the

sections are stained with eosin from 0.2 to 3 minutes,

depending on the thickness of the sections. They are

dehydrated in alcohols of increasing concentration,

starting from 70º to 96º, clarified in carbol-xylene,

xylene, and placed in a balm. Result: cell nuclei are

stained blue-violet, the cytoplasm is pink. The method

of luminescent microscopic examination [19].

Statistical analysis. The data obtained were statistically

processed on a Pentium IV personal computer using

the Microsoft Excel program. In addition, methods of

traditional variational parametric and nonparametric

statistics were used. To establish the reliability of the

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results obtained, the coefficient t - Student test was

used. Differences were considered significant if the

frequency for the studied trait did not exceed 5% (P

<0.05). Statistical processing of digital data was carried

out using the SPSS 16.0 and Statistica 6.0 for Windows

application programs. Means and standard deviations,

medians and interquartile intervals, as well as non-

parametric methods (Mann-Whitney, Wilcoxon,

Kruskal-Wallis tests,), were determined. Analysis of the

probability of occurrence of the studied outcome in a

certain period (survival) was performed according to

the method of E. Kaplan - P. Meier. Cox stepwise

regression analysis was used to identify several risk

factors for survival. Analysis of the accuracy and

practical value of prognostic factors and the validity of

the models were measured by the method of

concordant (c-statistic) statistics (estimation of the

area under the ROC curve).

Results. The div divweight before the experiment

varied from 220 to 250 g. Group 1 - intact animals (10

rats each), served as controls for groups 3 and 4. 2nd

group

–

the creation of an experimental model of a

diabetic foot, against the background of alloxan

diabetes; To do this, 10 rats were injected

intraperitoneally with 2% alloxan in an amount of 20 mg

/ 100 g. In this experimental group, in the 2nd

experimental group, 8 rats died in the first 3 days as a

result of hyperglycemic and hypoglycemic coma, which

amounted to 80%. When examining the level of glucose

in the blood with a glucometer of the remaining rats, it

was 33.3 mmol/l and may have been higher, since the

maximum range of the glucometer is 33.3 mmol/l. The

remaining 2 rats sat in the corner, there were no

reactions to external stimuli, they were sedentary

when picked up. The animals did not touch the food.

On the next day 4, the remaining rats died.

The second series of the second group of the

experimental model of diabetes mellitus was created

based on alloxan at a dose of 15 mg per 100 g from 10

rats. In this series of experiments, in the first 3 days the

lethality was 50% (5 rats). The glucose levels of the

survivors (5 rats) ranged from 29.8 to 33.3 mmol/l.

During the next 4 days, the remaining rats died.

3rd series of the experiment of the 2nd group -

administration of alloxan intraperitoneally at a dose of

12 mg per 100 g per 100 rats. During the next 72 hours,

no lethal outcome was observed in rats, the range of

blood glucose levels in rats varied between 15.5 - 17

mmol/L. In rats on the skin of the footpad pad of the

right hind paw, a full-thickness rectangular wound

measuring 2 mm × 5 mm was created with a scalpel.

Rats were randomly divided into 2 groups, each group

of 50 rats. So it was created 3

–

a control group on 50

rats and 4 experimental groups n=50 rats. In both

groups, until the end of the experiment (17 days), no

death was recorded.

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Visual inspection. The first signs of diabetes were

manifested in the form of a sharp increase in water

consumption of 70-80 ml, polyphagia, polyuria,

hyperglycemia. With alloxan-induced diabetes mellitus

in animals during the experiment, lethargy, apathy, low

activity, tarnishing and loss of coat, weight loss,

clouding of the pupil and sclera, small-point erosion in

the tails and limbs were noted. The wool of animals

normally has a peculiar luster and is usually adjacent to

the skin. In dynamic observation in rats of the

experimental group, by the seventh day, the condition

began to improve.

In the study of indicators characterizing the state of

various organs, for example, indicators of the state of

liver cells and the degree of their damage are the

activity of AST and ALT enzymes. In our studies, the

activity of these enzymes in the blood of animals in

both groups was significantly higher than in intact

animals (ALT-34U/l±1.ASTAsT-33.4 U/l±1.1), Although, it

should be noted that already after three injections of

the drug rheomannisol, in the animals of the

experimental group, the ALT and AST enzymes

recorded

low

numbers

(52.6±1.6;

48.4±1.4,

respectively) compared with the control group (82.8±

1.4, 86.3±1.5). By the 7th day in the control group ALT-

79±0.ASTAsT-79±1.5, which is 1.8 times more than in

the experimental group - ALT-44.7±0.94 AST AST-43,

3±1.0. In our study, in animals, the degree of elevation

of the levels of enzymes alanine transferase and

aspartate transferase indicates a pronounced violation

of the cellular structure of the liver. Recorded

activation of transaminases may indicate a violation of

the integrity of hepatocyte membranes, leading to an

increase in their permeability, and subsequently to the

death of liver cells. A decrease in the activities of both

enzymes (ALT, AST) followed the injections of

rheomannisol in the experimental gr, out and on the

10th and 14th days, the numbers (ALT-37.5±0.62, AST-

37.1±0.69;

ALT-35.3±

0.54,

AST-34.9

±

1.04,

respectively) indicate the normalization of the

functional capacity of the liver, while in the control

group, the activity of ALT and AST enzymes even on

days 10, 14 (ALT-75.5 ± 1.1, AST-74.4±1.6; ALT-57.2±1.2,

AST-53.4±1.3, respectively) 2 times higher than in the

experimental one, and remain at a high level until the

end of the experiment (Table 1 ).

Table 1. Biochemical parameters of animal blood in an experimental model of diabetic foot.

Indexes

Glucose,

mmol/l

ALT, U/l

AST, U/l

Urea,

mmol/l

Creatinine

, mkmol/l

Total

protein, g/l

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Group of

animals

1 day

Intact

5,8+0,19

34,0+1,0

33,4+1,1

5,1+0,20

61,5+2,0

74,1+1,2

Control

16,6±0,29

**

*

75,1±1,8

***

72,7±1,3

**

*

13,8±0,27

***

142,6±2,4

***

58,4±1,0

***

Main

15,2±0,43

**

*^

70,4±1,0

***

^

66,7±1,1

**

*^^

13,5±0,27

***

141,0±3,3

***

58,8±0,63

**

*

3 days

Control

15,4±0,28

**

*

82,8±1,4

***

86,3±1,5

**

*

15,0±0,40

***

145,7±1,8

***

55,5±0,73

**

*

Main

12,0±0,31

**

*^^^

52,6±1,6

***

^^^

48,4±1,4

**

*^^^

9,8±0,29

**

*^^^

97,6±2,1

**

*^^^

60,1±0,86

**

*^^^

7 days

Control

14,1±0,20

**

*

79,0±0,93

**

*

79,0±1,5

**

*

12,8±0,20

***

127,6±1,8

***

59,4±0,51

**

*

Main

9,0±0,37

***

^^^

44,7±0,94

**

*^^^

43,3±1,0

**

*^^^

7,2±0,30

**

*^^^

78,2±2,6

**

*^^^

66,0±1,4

***

^^^

10 days

Control

13,8±0,16

**

*

75,5±1,1

***

74,4±1,6

**

*

12,2±0,24

***

113,2±2,4

***

63,3±0,71

**

*

Main

7,3±0,21

***

^^^

37,5±0,62

*^

^^

37,1±0,69

*^^^

5,8±0,19

*^

^^

68,7±1,2

*^

^^

73,5±0,80

^^

^

14 days

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Note: *- significantly compared with the intact group (*-P<0,05; **-P<0,01; ***-P<0,001)

^ - significantly compared with the control group (^-P<0,05; ^^-P<0,01; ^^^-P<0,001)

One of the laboratory signs of the development of

renal dysfunction indicates the content of urea and

creatinine in the blood plasma, in the first days of the

experiments, in rats of the experimental and control

groups were almost 2.5 times (without significant

differences between these groups) higher than in the

intact group (tables No. 1). After 3-fold intraperitoneal

administration of the drug reomannisol, on the 3rd day,

the experimental group showed a noticeable decrease

in the values of urea (9.81±0.29) and creatinine

(97.6±2.1) by 1.5 times relative to the values control

group (urea-15.0±0.40; creatinine-145.7±1.8). On the

7th day in the groups of rats treated with reomannisol,

the levels of urea and serum creatinine (7.2±0.30 and

78.2±2.6, respectively) were lower compared to

control animals (12.8±0. 20 and 127.6±1.8, respectively)

by almost 1.7 times. On days 10, 14, urea values and

creatinine clearance (urin-5.8±0.19; creat-68.7±1.2;

urine-5.2±0.22; creat-63.8±1.3 respectively) in the

experimental group were close to those of the intact

group of rats (urea-5.1±0.20; creatinine-61.5±2.0).

However, in the control group, it was accompanied by

a higher value of urea and creatinine clearance, and on

the 14th day, they were urea-9.7±0.30 and creatinine-

96.7±1.6 - an average of 1.7 times higher than the values

of the experimental group (Table 1).

Evaluated at the end of the study on the background

of therapy with the studied preparations of

reomannisol, based on the results obtained, we can say

about the positive effect of the drug on renal activity,

as well as on protein metabolism.

Table 2. The product of POL is malonic dialdehyde (MDA).

Control

12,9±0,19

**

*

57,2±1,2

***

53,4±1,3

**

*

9,7±0,30

**

*

96,7±1,6

**

*

68,3±0,57

**

*

Main

6,5±0,13

*^^^

35,3±0,54

^^

^

34,9±1,04

^^^

5,2±0,22

^^

^

63,8±1,3

^^

^

75,8±0,63

^^

^

Days

Control group,

mkmol/l.

Main group, mkmol/l.

Intact group,

mkmol/l.

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)

(2023:

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)

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Note: *- significantly compared with the intact group (*-P<0,05; **-P<0,01; ***-P<0,001)

^ - significantly compared with the control group (^-P<0,05; ^^-P<0,01; ^^^-P<0,001)

Under the conditions of the model we have chosen,

the state of the LPO-MDA system was also studied

since this system is a key link in the pathogenesis of

diabetes mellitus. On the 1st day of the experiment, the

content of malondialdehyde was significantly higher in

both groups compared to intact rats (0.87 ± 0.02),

which indicates the formation of a large amount of lipid

peroxidation products, indicating the processes of

destruction of cell membranes (Table 2). The effect of

daily administration of reomannisol at a dose of 1

ml/100 g (experimental group) on the intensity of lipid

peroxidation on the 7th day was expressed by a

noticeable decrease in the content of MDA (1.02 ± 0.01)

by 1.2 times relative to the control group (1.27 ±0.01).

At the end of the experiment (day 14) in the group

receiving traditional treatment, the animals retained a

high level of MDA-1.17 ± 0.01, indicating a high content

of free radicals in the animal div. While in the

experimental group there is a stable decline in the level

of MDA and on the 10th, 14th day fixes a normal level

of MDA (respectively 0.93±0.01; 0.90±0.02). This result

indicates the antioxidant, detoxifying effect of the

drug reomannisol, which is characteristic of it.

MWM isolated from blood plasma and erythrocytes in

rats modeled with diabetes mellitus by alloxan can

activate LPO processes in the membranes of animal

erythrocytes. The state of endointoxication is

characterized, as a rule, by the activation of lipid

peroxidation, and they also act as a factor in the

aggravation of EI processes [7, 8].

Thus, judging from Table 3, high content of MWM

products, which cause the development of

endotoxemia, was found in the blood. It was revealed

that at the beginning of the experiment, the content of

MWM in blood plasma and erythrocytes in animals of

both groups was approximately 1.7-2 times higher than

in the intact group (see Table 3). It can also be said,

1

1,39±0,02

***

1,35±0,02

***

0,87±0,02

3

1,43±0,02

***

1,09±0,01

***^^^

-

7

1,27±0,01

***

1,02±0,01

***^^^

-

10

1,22±0,01

***

0,93±0,01

*^^^

-

14

1,17±0,01

***

0,90±0,02

^^^

-

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(2023:

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)

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reliably given by this table, that the numbers of the

toxemia index in plasma and erythrocytes are higher

than those in the intact group. The peptide component

of MWM is represented by the content of

oligopeptides in plasma and erythrocytes in both

groups, which also significantly exceeded by 1.6

–

2.4

times the value in the group of relatively intact animals.

This may indicate the activation of pathological

proteolysis processes. After the use of reomannisol,

the experimental group showed a tendency to reduce

all indicators of endogenous intoxication. By the 7th

day, the indices of MWM, OP of plasma (pl.) and

erythrocytes (eryt.) in the control group were on

average 1.2 times higher than those of the

experimental group. At 10, 14 days in the experimental

- fix the values of indicators corresponding to the intact

group and the normalization of the pathological

process in the div. Animals that received only

traditional treatment, EI indicators remain elevated on

average 1.2 times than in the experimental group, and

the state of intoxication persists until the end of the

experiment.

Table 3. Dynamics of change in indicators of endogenous intoxication.

Serum

Erythrocytes

Medium

weight

molecule

s

(MWM)

of

plasma,

Conv.

unit

Oligopeptid

es (OP) of

plasma, g/l

Toxemic

index (TI)

of plasma,

conv. unit

Intoxication

index (II)

conv. unit

Medium

weight

molecules

(MWM)

of eryt.,

conv. unit

Oligopeptid

es (OP) of

eryt., g/l

Toxemic

index (TI)

of eryt,

conv. unit

SCE, %

Intact
group

3,6±0,24

0,45±0,04

1,81±0,20

3,57±0,36

3,5±0,21

0,68±0,04

2,28±0,40

7,8±0,43

Contr
ol
group
Day 1

6,1±0,22

*

**

0,78±0,06

***

4,41±0,55

*

**

12,04±0,62

*

**

7,3±0,25

**

*

1,16±0,07

***

7,79±0,62

**

*

12,8±0,67

**

*

Main
group
Day 1

6,1±0,17

*

**

0,77±0,04

***

4,20±0,21

*

**

11,54±0,67

*

**

7,0±0,16

**

*

1,12±0,07

***

7,44±0,36

**

*

12,7±0,47

**

*

Contr
ol
group
Day 3

5,6±0,16

*

**

0,70±0,05

***

3,73±0,45

*

*

10,64±0,46

*

**

6,4±0,19

**

*

1,02±0,06

***

7,21±0,22

**

*

11,7±0,35

**

*

Main
group

5,3±0,09

*

**

0,69±0,05

**

3,36±0,28

*

**

8,71±0,99

**

*

5,9±0,08

**

*^

0,96±0,06

***

5,54±0,65

**

*^

10,4±0,44

**

*^

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(2023:

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)

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Day 4

Contr
ol
group
Day 7

5,3±0,11

*

**

0,67±0,05

**

3,09±0,22

*

**

8,51±0,35

**

*

5,6±0,11

**

*

0,92±0,05

**

5,79±0,32

**

*

9,6±0,31

**

Main
group
Day 7

4,0±0,11

^

^^

0,58±0,02

*

2,15±0,26

^

5,61±0,62

*^

^^

4,1±0,11

*^

^^

0,78±0,04

^

3,46±0,36

*^

^^

8,3±0,17

^^

Contr
ol
group
Day 10

4,9±0,10

*

**

0,56±0,03

*

2,83±0,23

*

*

6,84±0,31

**

*

5,2±0,11

**

*

0,85±0,05

*

4,64±0,23

**

*

9,3±0,21

**

Main
group
Day 10

3,7±0,14

^

^^

0,48±0,05

1,86±0,22

^

^

3,65±0,24

^^

^

3,7±0,12

^^

^

0,72±0,05

^

2,43±0,17

^^

^

8,0±0,23

^^^

Contr
ol
group
Day 14

4,2±0,11

*

0,52±0,03

2,39±0,15

*

5,56±0,24

**

*

4,2±0,10

**

0,77±0,04

3,30±0,16

*

8,7±0,17

*

Main
group
Day 14

3,5±0,18

^

^

0,45±0,04

1,80±0,23

^

3,55±0,37

^^

^

3,2±0,17

^^

^

0,68±0,02

2,30±0,22

^^

7,8±0,43

^

Note: *- significantly compared with the intact group (*-P<0,05; **-P<0,01; ***-P<0,001)

^ - significantly compared with the control group (^-P<0,05; ^^-P<0,01; ^^^-P<0,001).

The study of the sorption capacity of erythrocyte

membranes was carried out on erythrocytes from 10

practically healthy rats. The mean SCE in this group was

7.8% ± 0.43. After the administration of alloxan to the

div of rats, in both groups on the first days, a regular

increase in SCE was observed on average by 1.6 times,

intoxication index was 3.3 times that in the intact atop.

The redistribution of the toxic load between plasma

and blood erythrocytes is a necessary part of the

div's natural detoxification [2, 10]. Endotoxins bind

to the transmembrane protein of erythrocytes -

glycophorin, and in this form are transported to the

detoxification organs.

As a result, the use of reomannisol intraperitoneally in

rats of the experimental group improved the condition

of the animals, reduced the EI of the div. By 10, 14

days in the control group Intoxication index (II)

6.84±0.31; 5.56±0.24 and SCE 9.3±0.21; 8.7 ± 0.17,

respectively, were, on average, 1.7 (II) and 1.1 (SCE)

higher than the values of the experimental group - II

3.65 ± 0.24; 3.55±0.37 and SCE 8.0±0.23; 7.8±0.43 (see

table No. 3). This is due to the fact because the qualities

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of an antioxidant that improves blood rheology, a

detoxifying effect (enterosorbent), and a diuretic,

which have the effect of "biochemical sanitation" and

restores the physiological functions of cells for the

biotransport of endotoxins.

Wound healing is a big problem for diabetic patients.

This problem is observed both on a cellular and

humoral basis.

When examining the wound, the following parameters

of the course of the wound process were taken into

account: the presence and nature of the inflammatory

reaction, the presence and nature of the scab, the

strength of its adherence to the underlying tissues, the

severity of perifocal inflammation, skin hyperemia and

tissue infiltration in the wound area, the condition of

the edges and bottom of the wound, the timing of

wound cleansing from necrotic tissues and the

appearance of granulations, the nature of granulation

tissue, the timing of the onset of epithelization of

wounds. At 24 hours post-injury in both experimental

groups, the size of the wound increased in both groups

as the edges of the wounds were stretched further

apart due to edema, the edema spread to the entire

foot (Figure 1). Also, in both groups on the 2nd day

after the formation of a model of a rectangular skin

wound, it is observed that the surface of the wound

defect was covered with a thin scab formed by wound

discharge. When taking the animal in hand, the crust

was easily damaged, a transparent exudate leaked out.

Pronounced signs of inflammation are noted: the

edges of the wound are edematous, hyperemic with

areas of necrosis, the bottom of the wound is covered

with areas of fibrin.

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Figure 1. Images of foot wounds on days 1, 3 after injury and comparison of the size (area) of wounds between

control and experimental groups.

When analyzing the results of planimetric studies of

the speed epithelialization of wound defects, on the

3rd day of the experiment, there were no particular

differences in the groups. In both groups, on the 3rd

day, wound defects in animals were covered with a

dense dark-colored scab, inflammation persisted.

When viewed perifocally from the wound, bulging of

the skin was determined in both groups. But it should

be noted that during the revision of the wound in the

control group, the scab was easily removed from the

wound relative to the experimental group, under the

scab - the tissue was dull in places, there was a layer of

fibrin, there were areas of necrosis. Also, it should be

noted that the experimental group showed a decrease

in edema and hyperemia of the edges and walls of

wounds - it is on the decline, the beginning of the

formation of angiogenesis and elements of granulation

from the bottom of the wound can be traced,

compared with the control group.

Table 4. Comparative results of wound healing in animals with an experimental model of diabetic foot.

Control group

Main group

No

Wound size,

mm

Wound

area

mm

2

Popov

value

%

Wound size, mm

Wound

area mm

2

Popov

value %

1

2,0±0,

03

5,0±0,

02

10,1±0,

16

-

2,0±0,0

3

5,0±0,0

2

10,1±0,1

6

-

3

1,9±0,

02

4,7±0,

02

8,6±0,0

8

5,0±0,

27

1,7±0,0

2

***

4,5±0,0

2

***

7,4±0,05

*

**

8,9±0,46

**

*

7

1,7±0,

02

4±0,02 6,5±0,0

7

6,1±0,

30

1,5±0,0

2

***

3,0±0,0

2

***

4,3±0,05

*

**

10,3±0,18

*

**

10

1,6±0,

02

3,2±0,

02

4,9±0,0

5

8,4±0,

21

-

-

-

-

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Note: *- significantly compared with the control group (*-P<0,05; **-P<0,01; ***-P<0,001)

In the experimental group, the scab was difficult to

detach, tissues in places with a slight overlay of fibrin.

Swelling in the area of the foot wound continued in the

rats of the control group on the 7-8th day, but in the

rats of the experimental group, it decreased already on

the 5th day after the injury. From table 4 it follows that

on the 7th day after the injury in rats from the

experimental group when using the drug, there was a

significant decrease in the area of the wounds (4.3 ±

0.05 mm2) 2 times than its original wound, and 1.5

times than in rats of the control group (6.5±0.07 mm2),

due to wound contraction and marginal epithelization

(Figure 6). The crust from the wound was removed

with great difficulty, under it there was a brightly

granulating wound defect with pronounced signs of

marginal epithelization, far ahead of the control group.

Also, in the rats of the experimental group, almost

complete closure of the wound defect is observed, it is

noted that the wound is bleeding well, this indicates an

improvement in blood circulation in the wound, which

exceeds this indicator over the control group. When

examining the histological section of the wound under

a microscope, there is a limitation and rejection of the

destructive-necrotic tissue on the surface of the

wound (Figure 3). At the same time, in the

circumference of the wound, the tissue of the

epidermis is compacted and the focus of destruction of

the dermis is delimited from the underlying healthy

elements of the tissue of the dermis. As part of the

destructive tissue, the development of the process of

disintegration and disorganization of both cellular and

fibrous structures is determined. In the underlying

connective tissue of the dermis, a neoplasm of hair

follicles, compaction of fibrous structures and an

increase in the proliferative activity of histiocytic cells

are determined.

Figure 2. Control group, Day 7. Diabetic wound. Preservation of necrotic mass and inflammatory infiltrate in the

bottom of the diabetic foot. Staining: hematoxylin-eosin. Magnification: 10x40.

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184

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Figure 3. Main group, Day 7. Rejection of necrotic tissue on the surface of a diabetic wound. Staining: hematoxylin-

eosin. Magnification: 10x40.

Figure 4. Control group, Day 10. Diabetic wound. Formation of a dense inflammatory infiltrates around the wound

of a diabetic foot. Staining: hematoxylin-eosin. Magnification: 10x40.

Figure 5. Main group, day 10. Compaction of the surface layers of the epidermis, fibrosis of the connective tissue of

the dermis. Staining: hematoxylin-eosin. Magnification: 10x40.

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On the 7th day after treatment with the traditional

method of an experimental model of a diabetic foot in

the control group, at the bottom and circumference of

the diabetic wound, necrobiotic tissue and acute

inflammatory infiltrate are preserved in the form of a

structureless tissue mass, in the circumference of

which it is infiltrated with leukocyte cells, and a picture

of the formation of poorly differentiated (granulation)

is also found. tissue, the process of vasculogenesis is

very weak (Figure 2). As part of the structureless mass,

there are foci of edema and tissue vacuolization, as

well as hematoxylin conglomerates and calcification.

Thus,

the

development

of

microangiopathy

phenomena took place, which makes it possible to

consider diabetic microangiopathy as one of the

morphological and functional manifestations of

diabetes mellitus.

Figure 6. Images of foot wounds on days 7, 10, 14 after injury and comparison of the size (area) of wounds between

control and experimental groups.

By the 10th day in the experimental group, who

received traditional treatment and Reomanisol, an

independent almost complete closure of the wound

defect and hair growth around the wound were noted

(Figure 6). There is a rejection of the necrotic part of

the epidermal tissue, dedifferentiation of the

remaining part of the stratified epithelium in the form

of compaction of the surface layers, vacuolization, and

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an increase in the proliferative activity of the cells of

the basal layers (Figure 5). The connective tissue of the

dermis is compacted, without signs of an acute

inflammatory process, the fibrous structures are

transformed into dense, homogeneous, fibrous

masses due to disorganization and fusion with each

other. In them, cellular structures are localized along

the periphery and around the vessels, and they are in a

proliferative active state. On the 10th day after the

treatment of diabetic foot with reomannisol,

regeneration

of

the

integumentary

stratified

epithelium is noted in the form of sliding of epithelial

cells onto the surface of the wound. At the same time,

the epidermis is represented in the regeneration zone

by several layers of active and hyperchromic

epitheliocytes. Under the epidermis, the formation of

a basement membrane from loose fibrous structures is

determined. In the tissue of the dermis, the presence

of foci of reparative regeneration is determined in the

form of excessive formation of fibrous, cellular

structures that differ from the surrounding tissue by

the presence of many vessels and proliferatively active

histiocytic cells. Both in the epidermis and the dermis,

there are no signs of an acute inflammatory process.

In the control group, on the 10th day, a wound defect

of about 4.9 ± 0.05 mm2 remains (Figure 6). At the

bottom and in the circumference of the wound, the

formation of inflammatory granulation tissue with foci

of necrosis and hemorrhage is noted. The

inflammatory infiltrate is represented by proliferatively

active lymphoid and histiocytic cells (Figure 4),

randomly arranged fibrous structures consisting of

argyrophilic and collagen fibers. In the center of the

inflammatory infiltrate, a defect surrounded by

fibrinoid necrosis and a homogeneous fibrous mass is

determined. In the circumference of the inflammatory

infiltrate, the connective tissue is subjected to edema,

loosening with the breakdown of fibrous structures,

and cell necrobiosis. The wound healed on the 14th day

of the experiment (Figure 6). Thus, hyperglycemia

causes microvascular complications due to impaired

angiogenesis, which leads to a prolongation of the

inflammatory effect of the wound and the period of

wound healing.

The use of standard wound treatments (iodine and

levomekol) and the drug reomanisol, indicators of

planimetric control ovethroughoute the wound

process in animals of this group (experimental) are at

a consistently high level.

CONCLUSIONS

1. The best option for creating an experimental model

of a diabetic foot is the introduction of alloxan

intraperitoneally in a single dose of 12 mg per 100 g, in

which moderate diabetes develops.

2. After using the drug reomannisol intraperitoneally at

a dose of 1 ml / 100 g 1 time per day for 5 days, there

was a sharp decline in EI numbers. On the 10th day, the

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5.

694

)

(2022:

5.

893

)

(2023:

6.

184

)

OCLC

–

1121105677

Publisher:

Oscar Publishing Services

Servi

EI values in the experimental group returned to

normal, similar to those in the intact group. The drug

reomannisol performs "biochemical rehabilitation",

due to its inherent qualities: antioxidant, improves

blood rheology, detoxification, and diuretic. In rats of

the control group, the EI numbers remain at high levels

until the end of the experiment.

3. The results of biochemical studies demonstrate

positive dynamics in experimental animals with a

diabetic foot model when using the drug reomannisol.

This was manifested by the fact that by the 10th day

there was a decrease and normalization of the level of

glucose in the peripheral blood, indicators of renal

clearance (urea, creatinine), liver (ALT, AST, albumins).

4. An open, full-thickness wound of the foot, in rats

with DM, had low blood circulation, prolonged

inflammation, and was characterized by a violation of

the inflammatory and proliferative phases of the

healing

process,

which

is

associated

with

hyperglycemia. Thus, this model of the open foot in

rats provides a good approach for studying the process

of wound healing in DM, and this model can be

regarded as creating an analog of the human diabetic

foot syndrome in an experimental model of alloxan-

induced diabetes mellitus.

5. The rate of healing of wound defects in rats with

diabetic foot syndrome in the control group falls on the

14th day, since the terms of resorption and rejection of

necrotic tissues in the wound are lengthened, damage

to

the

vessels

of

the

microvasculature

(microangiopathy), edema is observed for a long time.

The wounding process against the background of DM

is characterized by the late formation of angiogenesis,

slowing down and impaired maturation of granulation

tissue, marginal epithelialization. In the experimental

group, in rats, along with the local traditional method

of wound treatment, the drug reomannisol was used

intraperitoneally, as a result, wound healing was

recorded on the 10th day from the moment the wound

was applied to the foot of the rats. The use of local

treatment and reomannisol can enhance angiogenesis

in the early stages of the experiment and restore

disturbed microcirculation (neoplasms of blood

vessels), increase macrophage response, fibroblast

proliferation,

maturation

and

remodeling

of

granulation tissue and its epithelization, reduce the

inflammatory reaction, which leads to more effective

and early healing wound area.

6. Comprehensive treatment (application of a local

traditional method of treatment on the wound and the

drug reomannisol) in an experimental model of the

diabetic foot have positive effects on reparative

processes and wound healing, due to the formation

and enhancement of angiogenesis, as well as on the

functional parameters of vital organs by reducing

intoxication organism.

Volume 03 Issue 11-2023

85

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(ISSN

–

2771-2265)

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03

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)

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Servi

Ethical approval. Operations and all manipulations with

animals were carried out using general anesthesia, in

compliance with the principles of humanity outlined in

the

directives

of

the

European

Community

(86/609/EEC) and the Declaration of Helsinki, by the

"Rules for working with experimental animals". The

ethical approval for the study was granted by Tashkent

Medical Academy and the Committee of Ethical

Approval for Researches under the Ministry of Health

of the Republic of Uzbekistan.

Conflict of interest. The authors declare that they have

no competing interests.

Funding.

No funding sources to declare.

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