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<article article-type="research-article" dtd-version="1.3" xmlns:mml="http://www.w3.org/1998/Math/MathML" xmlns:xlink="http://www.w3.org/1999/xlink" xmlns:xsi="http://www.w3.org/2001/XMLSchema-instance" xml:lang="en"><front><journal-meta><journal-id journal-id-type="publisher-id">vetpatol</journal-id><journal-title-group><journal-title xml:lang="en">Russian Journal of Veterinary Pathology</journal-title><trans-title-group xml:lang="ru"><trans-title>Ветеринарная патология</trans-title></trans-title-group></journal-title-group><issn pub-type="epub">2949-4826</issn><publisher><publisher-name>Don State Technical University</publisher-name></publisher></journal-meta><article-meta><article-id pub-id-type="doi">10.23947/2949-4826-2025-24-4-43-54</article-id><article-id custom-type="elpub" pub-id-type="custom">vetpatol-2090</article-id><article-categories><subj-group subj-group-type="heading"><subject>Research Article</subject></subj-group><subj-group subj-group-type="section-heading" xml:lang="en"><subject>ANIMAL PATHOLOGY, MORPHOLOGY, PHYSIOLOGY, PHARMACOLOGY AND TOXICOLOGY</subject></subj-group><subj-group subj-group-type="section-heading" xml:lang="ru"><subject>ПАТОЛОГИЯ ЖИВОТНЫХ, МОРФОЛОГИЯ, ФИЗИОЛОГИЯ, ФАРМАКОЛОГИЯ И ТОКСИКОЛОГИЯ</subject></subj-group></article-categories><title-group><article-title>A Study on Morphofunctional State of Djungarian Hamster (Phodopus Sungorus) Lungs  and Main Organs of Detoxification under Long-Term Exposure to E-Cigarette Aerosol</article-title><trans-title-group xml:lang="ru"><trans-title>Исследование морфофункционального состояния легких и центральных органов детоксикации джунгарских хомячков (Phodopus sungorus)  при длительном воздействии аэрозоля электронных сигарет</trans-title></trans-title-group></title-group><contrib-group><contrib contrib-type="author" corresp="yes"><contrib-id contrib-id-type="orcid">https://orcid.org/0000-0002-5076-2113</contrib-id><name-alternatives><name name-style="eastern" xml:lang="ru"><surname>Сахаров</surname><given-names>А. В.</given-names></name><name name-style="western" xml:lang="en"><surname>Sakharov</surname><given-names>A. V.</given-names></name></name-alternatives><bio xml:lang="ru"><p>Андрей Валентинович Сахаров, доктор биологических наук, доцент, заведующий кафедрой биологии и экологии</p><p>630126, г. Новосибирск, ул. Вилюйская, 28</p></bio><bio xml:lang="en"><p>Andrey V. Sakharov, Dr.Sci.(Biology), Associate Professor, Head of the Biology and Ecology, Department</p><p>28, Vilyuyskaya Str., Novosibirsk, 630126</p></bio><xref ref-type="aff" rid="aff-1"/></contrib><contrib contrib-type="author" corresp="yes"><contrib-id contrib-id-type="orcid">https://orcid.org/0000-0001-7137-2424</contrib-id><name-alternatives><name name-style="eastern" xml:lang="ru"><surname>Бырдина</surname><given-names>В. И.</given-names></name><name name-style="western" xml:lang="en"><surname>Byrdina</surname><given-names>V. I.</given-names></name></name-alternatives><bio xml:lang="ru"><p>Виталина Игоревна Бырдина, кандидат биологических наук, доцент кафедры биологии и экологии Института естественных и социально-экономических наук </p><p>630126, г. Новосибирск, ул. Вилюйская, 28</p></bio><bio xml:lang="en"><p>Vitalina I. Byrdina, Cand.Sci.(Biology), Associate Professor of the Biology and Ecology Department of the Institute of Natural and Socio-Economic Sciences</p><p>28, Vilyuyskaya Str., Novosibirsk, 630126</p></bio><xref ref-type="aff" rid="aff-1"/></contrib><contrib contrib-type="author" corresp="yes"><name-alternatives><name name-style="eastern" xml:lang="ru"><surname>Задубровский</surname><given-names>П. А.</given-names></name><name name-style="western" xml:lang="en"><surname>Zadubrovsky</surname><given-names>P. A.</given-names></name></name-alternatives><bio xml:lang="ru"><p>Павел Александрович Задубровский, кандидат биологических наук, старший научный сотрудник Лаборатории структуры и динамики популяций позвоночных животных; преподаватель кафедры биологии и экологии </p><p>630126, г. Новосибирск, ул. Вилюйская, 28</p><p>630091, г. Новосибирск, ул. Фрунзе, 11</p></bio><bio xml:lang="en"><p>Pavel A. Zadubrovsky, Cand.Sci.(Biology), Senior Research Associate at the Laboratory of Structure and Dynamics of Vertebrate Animal Populations, Lecturer of the Biology and Ecology  Department </p><p>28, Vilyuyskaya Str., Novosibirsk, 630126</p><p>11, Frunze Str., Novosibirsk, 630091</p></bio><email xlink:type="simple">etolog@mail.com</email><xref ref-type="aff" rid="aff-2"/></contrib><contrib contrib-type="author" corresp="yes"><contrib-id contrib-id-type="orcid">https://orcid.org/0000-0001-6941-7566</contrib-id><name-alternatives><name name-style="eastern" xml:lang="ru"><surname>Задубровская</surname><given-names>И. В.</given-names></name><name name-style="western" xml:lang="en"><surname>Zadubrovskaya</surname><given-names>I. V.</given-names></name></name-alternatives><bio xml:lang="ru"><p>Инна Валерьевна Задубровская, кандидат биологических наук, старший научный сотрудник Лаборатории структуры и динамики популяций позвоночных животных; доцент кафедры биологии и экологии </p><p>630126, г. Новосибирск, ул. Вилюйская, 28</p><p>630091, г. Новосибирск, ул. Фрунзе, 11</p></bio><bio xml:lang="en"><p>Inna V. Zadubrovskaya, Cand.Sci. (Biology), Senior Research Associate at the Laboratory of Structure and Dynamics of Vertebrate Animal Populations; Associate Professor of the Biology and Ecology Department </p><p>28, Vilyuyskaya Str., Novosibirsk, 630126</p><p>11, Frunze Str., Novosibirsk, 630091</p></bio><email xlink:type="simple">inna_zadubrovskaya@mail.ru</email><xref ref-type="aff" rid="aff-2"/></contrib><contrib contrib-type="author" corresp="yes"><contrib-id contrib-id-type="orcid">https://orcid.org/0000-0002-8435-7482</contrib-id><name-alternatives><name name-style="eastern" xml:lang="ru"><surname>Потапова</surname><given-names>О. Ф.</given-names></name><name name-style="western" xml:lang="en"><surname>Potapova</surname><given-names>O. F.</given-names></name></name-alternatives><bio xml:lang="ru"><p>Ольга Федоровна Потапова, научный сотрудник Лаборатории структуры и динамики популяций позвоночных животных </p><p>630091, г. Новосибирск, ул. Фрунзе, 11</p></bio><bio xml:lang="en"><p>Olga F. Potapova, Research Associate at the Laboratory of Structure and Dynamics of Vertebrate Animal Populations</p><p>11, Frunze Str., Novosibirsk, 630091</p></bio><email xlink:type="simple">ofpotapova@yandex.ru</email><xref ref-type="aff" rid="aff-3"/></contrib><contrib contrib-type="author" corresp="yes"><contrib-id contrib-id-type="orcid">https://orcid.org/0000-0001-8672-7216</contrib-id><name-alternatives><name name-style="eastern" xml:lang="ru"><surname>Кондратюк</surname><given-names>Е. Ю.</given-names></name><name name-style="western" xml:lang="en"><surname>Kondratyuk</surname><given-names>E. Yu.</given-names></name></name-alternatives><bio xml:lang="ru"><p>Екатерина Юрьевна Кондратюк, кандидат биологических наук, научный сотрудник </p><p>630117, г. Новосибирск, ул. Арбузова, 6</p></bio><bio xml:lang="en"><p>Ekaterina Yu. Kondratyuk, Cand.Sci.(Biology), Research Associate </p><p>6, Arbuzov Str., Novosibirsk, 630117</p></bio><xref ref-type="aff" rid="aff-4"/></contrib><contrib contrib-type="author" corresp="yes"><name-alternatives><name name-style="eastern" xml:lang="ru"><surname>Бондаренко</surname><given-names>С. С.</given-names></name><name name-style="western" xml:lang="en"><surname>Bondarenko</surname><given-names>S. S.</given-names></name></name-alternatives><bio xml:lang="ru"><p>Сергей Сергеевич Бондаренко, аспирант </p><p>190013, г. Санкт-Петербург, Московский пр., 24–26/49</p></bio><bio xml:lang="en"><p>Sergey S. Bondarenko, Postgraduate Degree Student</p><p>24–26/49, Moskovsky Ave., St. Petersburg, 190013</p></bio><email xlink:type="simple">cergeib@mail.ru</email><xref ref-type="aff" rid="aff-5"/></contrib><contrib contrib-type="author" corresp="yes"><contrib-id contrib-id-type="orcid">https://orcid.org/0000-0002-0944-5394</contrib-id><name-alternatives><name name-style="eastern" xml:lang="ru"><surname>Новиков</surname><given-names>Е. А.</given-names></name><name name-style="western" xml:lang="en"><surname>Novikov</surname><given-names>E. A.</given-names></name></name-alternatives><bio xml:lang="ru"><p>Евгений Анатольевич Новиков, доктор биологических наук, заведующий Лабораторией структуры и динамики популяций позвоночных животных; заведующий кафедрой экологии </p><p>630091, г. Новосибирск, ул. Фрунзе, 11</p><p>630039, г. Новосибирск, ул. Добролюбова, 160</p></bio><bio xml:lang="en"><p>Evgeny A. Novikov, Dr.Sci. (Biology), Head of the Laboratory of Structure and Dynamics of Vertebrate Animal Populations; Head of the  Ecology Department</p><p>11, Frunze Str., Novosibirsk, 630091</p><p>160, Dobrolyubova Str., Novosibirsk, 630039</p></bio><email xlink:type="simple">eug-nov5@yandex.ru</email><xref ref-type="aff" rid="aff-6"/></contrib></contrib-group><aff-alternatives id="aff-1"><aff xml:lang="ru"><institution>Новосибирский государственный педагогический университет</institution><country>Россия</country></aff><aff xml:lang="en"><institution>Novosibirsk State Pedagogical University</institution><country>Russian Federation</country></aff></aff-alternatives><aff-alternatives id="aff-2"><aff xml:lang="ru"><institution>Новосибирский государственный педагогический университет;&#13;
Институт систематики и экологии животных СО РАН</institution><country>Россия</country></aff><aff xml:lang="en"><institution>Novosibirsk State Pedagogical University;&#13;
Institute of Systematics and Ecology of Animals, Siberian Branch of Russian Academy of Sciences</institution><country>Russian Federation</country></aff></aff-alternatives><aff-alternatives id="aff-3"><aff xml:lang="ru"><institution>Институт систематики и экологии животных СО РАН</institution><country>Россия</country></aff><aff xml:lang="en"><institution>Institute of Systematics and Ecology of Animals, Siberian Branch of Russian Academy of Sciences</institution><country>Russian Federation</country></aff></aff-alternatives><aff-alternatives id="aff-4"><aff xml:lang="ru"><institution>Научно-исследовательский институт клинической и экспериментальной лимфологии – филиал ФГБНУ &#13;
«ФИЦ ИЦиГ СО РАН»</institution><country>Россия</country></aff><aff xml:lang="en"><institution>Research Institute of Clinical and Experimental Lymрhology – Branch of Institute of Cytology and Genetics, Siberian Branch of Russian Academy of Sciences</institution><country>Russian Federation</country></aff></aff-alternatives><aff-alternatives id="aff-5"><aff xml:lang="ru"><institution>Санкт-Петербургский государственный технологический институт</institution><country>Россия</country></aff><aff xml:lang="en"><institution>Saint Petersburg State Institute of Technology</institution><country>Russian Federation</country></aff></aff-alternatives><aff-alternatives id="aff-6"><aff xml:lang="ru"><institution>Институт систематики и экологии животных СО РАН;&#13;
Новосибирский государственный аграрный университет</institution><country>Россия</country></aff><aff xml:lang="en"><institution>Institute of Systematics and Ecology of Animals, Siberian Branch of Russian Academy of Sciences;&#13;
Novosibirsk State Agrarian University</institution><country>Russian Federation</country></aff></aff-alternatives><pub-date pub-type="collection"><year>2025</year></pub-date><pub-date pub-type="epub"><day>19</day><month>01</month><year>2026</year></pub-date><volume>24</volume><issue>4</issue><fpage>43</fpage><lpage>54</lpage><permissions><copyright-statement>Copyright &amp;#x00A9; Sakharov A.V., Byrdina V.I., Zadubrovsky P.A., Zadubrovskaya I.V., Potapova O.F., Kondratyuk E.Y., Bondarenko S.S., Novikov E.A., 2025</copyright-statement><copyright-year>2025</copyright-year><copyright-holder xml:lang="ru">Сахаров А.В., Бырдина В.И., Задубровский П.А., Задубровская И.В., Потапова О.Ф., Кондратюк Е.Ю., Бондаренко С.С., Новиков Е.А.</copyright-holder><copyright-holder xml:lang="en">Sakharov A.V., Byrdina V.I., Zadubrovsky P.A., Zadubrovskaya I.V., Potapova O.F., Kondratyuk E.Y., Bondarenko S.S., Novikov E.A.</copyright-holder><license license-type="creative-commons-attribution" xlink:href="https://creativecommons.org/licenses/by/4.0/" xlink:type="simple"><license-p>This work is licensed under a Creative Commons Attribution 4.0 License.</license-p></license></permissions><self-uri xlink:href="https://www.vetpat.ru/jour/article/view/2090">https://www.vetpat.ru/jour/article/view/2090</self-uri><abstract><sec><title>Introduction</title><p>Introduction. The liquids of electronic nicotine delivery systems (ENDS), which have the multi-component composition, represent a major environmental hazard, as they contain extremely toxic substances. Although the popularity of this form of smoking grows, the data on the biological effects of long-term exposure of animals and humans to e-cigarette and vape components are insufficient. The aim of the present study is to investigate the morphofunctional state of the lungs and main organs of detoxification in Djungarian hamsters under long-term exposure to ENDS aerosol.</p></sec><sec><title>Materials and Methods</title><p>Materials and Methods. The research was conducted in 2021 in the colony of laboratory Djungarian hamsters kept at the Institute of Systematics and Ecology of Animals SA RAS. Thirty-six hamsters were divided into two groups. During 80 days, animals in the experimental group (10 females and 10 males) were exposed to vapour from heating the X-3 Yoghurt Pear liquid. The procedure was performed twice a day for 10 minutes, with a 2-hour interval. Hamsters in the control group (8 males and 8 females) were placed in exposure chambers but were not exposed to vapour. At the end of the 80-day experiment, the animals were decapitated, and organs were collected for preparing thin histological sections. The specimens were stained with Boehmer’s hematoxylin and eosin. Collagen distribution was determined using the Mallory method. Histological specimens of organs were examined under transmission light microscope</p></sec><sec><title>Results</title><p>Results. In experimental animals exposed to toxic vapour, a homogeneous black substance was detected in bronchial epithelial cells and in the alveolar interstitium. In the lung parenchyma, signs of developing interstitial pneumonia, atelectasis, emphysema, and obstructive bronchitis were detected, indicating impaired ventilation-perfusion relationships in the lung tissue and gas exchange disorder. In the kidneys, the homogeneous substance was localized in the lumen of renal tubules. Light optical microscopy revealed the main signs of lethal damage in renal epithelial cells. Strongly expressed dilation of the renal glomerular capillaries, coupled with a nearly 2-fold reduction in the surface area of renal corpuscles compared to control samples, indicates impaired hemodynamics and disrupted renal reabsorption-filtration function. Regarding the liver, a high level of localization of evolutionarily adapted to detoxification dark hepatocytes dying by apoptosis in the centrilobular region of the lobule, indicates the involvement of toxic substances in this process, which enter the liver with the blood.</p><p>Discussion and Conclusion. The experiment demonstrated the general pathogenic effects of ENDS aerosol on the lungs and organs of detoxification in animals after long-term exposure to it. Such studies are necessary in the context of the observed growth of consumption of the nicotine delivery systems at the global market. </p></sec></abstract><trans-abstract xml:lang="ru"><sec><title>Введение</title><p>Введение. Многокомпонентный состав жидкостей для электронных систем доставки никотина (ЭСДН) представляет большую опасность для экологии, так как содержит чрезвычайно токсичные вещества. Несмотря на растущую популярность этого вида курения, данных о биологических эффектах длительного влияния состава электронных сигарет и вейпов на организм животных и человека недостаточно. Цель настоящей работы — исследовать морфофункциональное состояние легких и центральных органов детоксикации джунгарских хомячков при длительном воздействии аэрозоля ЭСДН.</p></sec><sec><title>Материалы и методы</title><p>Материалы и методы. Работа выполнена в 2021 г. на лабораторной колонии джунгарского хомячка, содержащейся на базе ИСиЭЖ СО РАН. 36 хомячков разделили на две группы. Животных опытной группы (10 самок и 10 самцов) в течение 80 дней подвергали воздействию пара, полученного при нагревании жидкости X-3 Yoghurt Pear. Процедуру проводили каждый день в течение 10 мин, по 2 раза с интервалом в 2 ч. Хомячков контрольной группы (8 самцов и 8 самок) помещали в затравочные камеры, но не подвергали воздействию пара. По завершении 80 дней эксперимента производили декапитацию животных и забор органов для изготовления микросрезов. Обзорные препараты окрашивали гематоксилином Бемера и эозином. Распределение коллагена определяли по методу Маллори. Гистологические препараты органов изучали в проходящем свете с помощью микроскопа.</p></sec><sec><title>Результаты исследования</title><p>Результаты исследования. У животных опытной группы в результате экспозиции токсичным паром выявлено наличие гомогенного вещества черного цвета среди клеток эпителия бронхов и в интерстиции альвеолярных мешочков. В паренхиме легкого обнаружены признаки развивающейся интерстициальной пневмонии, ателектаза и эмфиземы, обструктивного бронхита, что свидетельствует о нарушении вентиляционно-перфузионных отношений в легочной ткани и газообмена. В почках локализация гомогенного вещества отмечена в просвете канальцев нефрона. На светооптическом уровне основные признаки летального повреждения характерны для клеток нефротелия. Ярко выраженная дилатация капилляров почечного клубочка в совокупности со снижением площади почечных телец практически в 2 раза, по сравнению с контрольными образцами, указывает на нарушение гемодинамики и реабсорбционно-фильтрационной функции почек. В печени высокий уровень локализации гибнущих апоптозом темных гепатоцитов центролобулярной зоны дольки, эволюционно приспособленных к детоксикации, указывает на причастность к этому процессу токсических веществ, поступающих в печень с кровью.</p></sec><sec><title>Обсуждение и заключение</title><p>Обсуждение и заключение. В ходе эксперимента доказано общепатогенное воздействие аэрозоля ЭСДН на легкие и органы детоксикации животных при длительном применении. Подобные исследование необходимы в условиях наблюдающегося роста потребления данных средств доставки никотина на мировом рынке.</p></sec></trans-abstract><kwd-group xml:lang="ru"><kwd>электронные системы доставки никотина</kwd><kwd>ЭСДН</kwd><kwd>аэрозоль электронных сигарет</kwd><kwd>вейпы</kwd><kwd>джунгарские хомячки</kwd><kwd>длительное воздействие</kwd><kwd>морфофункциональные изменения</kwd><kwd>лёгкие и органы детоксикации</kwd><kwd>почечная недоста-точность</kwd><kwd>апоптоз гепатоцитов</kwd></kwd-group><kwd-group xml:lang="en"><kwd>electronic nicotine delivery systems</kwd><kwd>ENDS</kwd><kwd>e-cigarette aerosol</kwd><kwd>vapes</kwd><kwd>Djungarian hamsters</kwd><kwd>long-term exposure</kwd><kwd>morphofunctional changes</kwd><kwd>lungs and organs of detoxification</kwd><kwd>renal failure</kwd><kwd>hepatocyte apoptosis</kwd></kwd-group><funding-group><funding-statement xml:lang="ru">Работа выполнена в рамках Федеральной программы фундаментальных научных исследований на 2021–2025 гг. FWGS -2021-0003.</funding-statement><funding-statement xml:lang="en">The work was carried out in the frame of the Federal Program for Fundamental Scientific Research for 2021–2025 FWGS-2021-0003.</funding-statement></funding-group></article-meta></front><body><p>Introduction. Electronic nicotine delivery systems (ENDS) first became widely available in Europe in 2006 and turned into the most popular alternative to conventional cigarettes [1–6], especially among young people and adolescents of the age of 14 and older [<xref ref-type="bibr" rid="cit1">1</xref>][7–10]. The most hazardous for the environment are the multi-component electronic cigarette (EC) liquids, which contain more than 30 toxic chemicals, including carbonyl compounds (aldehydes, ketones), metals, propylene glycol, and glycerol [11–16]. Moreover, carbonyl compounds include extremely toxic substances such as acrolein (maximum permissible concentration (MPC) in air 0.03 mg/m³) and formaldehyde (MPC 0.05 mg/m³), which irritate the mucous membranes of internal organs, as a minimum [<xref ref-type="bibr" rid="cit17">17</xref>]. Also, acrolein causes mutagenesis in bacteria and yeast, exhibits mutagenic properties in mammalian cell cultures, and reduces activity of some components of the immune defence [<xref ref-type="bibr" rid="cit18">18</xref>].</p><p>Studies examining the effects of two essential components of ENDS—propylene glycol and glycerin—show that propylene glycol, when aerosolized into the alveoli, boosts the destruction of surfactant, which ensures lung compliance and prevents lung tissue adhesion. This effect leads to pulmonary collapse (atelectasis), while adjacent areas undergo compensatory overstretching, causing emphysema. Propylene glycol is also considered a stimulating factor in the formation of squamous cell metaplasia of the larynx. In rats subjected to inhaling glycerin vapour, metaplasia of epiglottal epithelium was observed [<xref ref-type="bibr" rid="cit19">19</xref>]. It is also known that glycerin heated in an e-cigarette up to 500°C transforms into acrolein mentioned above.</p><p>Apart from the main components, the ENDS also use a variety of flavouring agents. The Generally Recognized as Safe (GRAS) list includes flavouring agents for ingestion, however, the number of studies on inhaling the aerosols containing such substances is few. For example, it has been proven that inhalation of diacetyl contained in e-liquid causes obliterating bronchiolitis, the so-called “popcorn lung” disease (the phenomenon was identified in the early 2000s due to the mass illnesses of workers of popcorn factories) [<xref ref-type="bibr" rid="cit20">20</xref>]. At some factories, diacetyl was replaced by acetylpropionyl, but even then, researchers from the US National Institute for Occupational Safety and Health (NIOSH) had to note significant deviations in the spirometry readings of workers at such factories [<xref ref-type="bibr" rid="cit21">21</xref>][<xref ref-type="bibr" rid="cit22">22</xref>]. In ENDS, these substances are used to impart buttery or caramel flavour, although pulmonary toxicity of acetylpropionyl to mammals has been proven. For example, rats exposed to it developed fibrosis and necrosis of the respiratory tract tissue; in mice exposed to the inhalation test (methacholine challenge test) more severe bronchoconstriction was observed [<xref ref-type="bibr" rid="cit23">23</xref>]. On the whole, despite more than 7000 ENDS flavours resulting from the range of flavouring agents available on the market [<xref ref-type="bibr" rid="cit24">24</xref>], only three studies have been published on the effects of flavouring agents on the organism [<xref ref-type="bibr" rid="cit15">15</xref>][<xref ref-type="bibr" rid="cit25">25</xref>][<xref ref-type="bibr" rid="cit26">26</xref>].</p><p>A considerable amount of information can be found in the literature on the effects of electronic cigarettes and vapes on the organism of mammals. For example, it has been proven that exposure to ENDS vapour altered pulmonary function in rats [<xref ref-type="bibr" rid="cit27">27</xref>]; reduced the conductivity of ion channels in sheep bronchial epithelial cells, and also led to mucus hyperconcentration [<xref ref-type="bibr" rid="cit28">28</xref>]. A significant increase in pro-inflammatory cytokines was recorded in the lungs of rats [<xref ref-type="bibr" rid="cit29">29</xref>], as well as development of the lipoid pneumonia [<xref ref-type="bibr" rid="cit30">30</xref>]. It was also found that steaming with nicotine-free liquid affected the vital organs, which manifested in interalveolar septa thickening in the lungs of rats, filling the bronchial tubes with mucus obstructing the lumen, and lymphoid infiltration in bronchial tubes. In the kidneys, a threefold expansion of the lumens in the Shumlyansky-Bowman capsules was recorded, along with the damage of the renal corpuscles and the epithelium of the proximal tubules [<xref ref-type="bibr" rid="cit31">31</xref>]. It was noted that numbers of bronchitis, pneumonia, and lung cancer have increased in dogs in large cities [<xref ref-type="bibr" rid="cit32">32</xref>]. Several studies revealed the hepatotoxicity of e-cigarette liquids in rats [<xref ref-type="bibr" rid="cit33">33</xref>]. However, the information on the biological effects of long-term use of e-cigarettes and vapes is insufficiently presented in the scientific literature.</p><p>The aim of the present study is to investigate the morphofunctional changes in the lungs and main organs of detoxification of Djungarian hamsters (Phodopus sungorus) during long-term exposure to e-cigarette and vape aerosols.</p><p>Materials and Methods. The research was conducted in 2021 at the Institute of Systematics and Ecology of Animals, Siberian Branch of Russian Academy of Sciences and the Experimental and Applied Biology Research and Educational Centre of Novosibirsk State Pedagogical University. The work was performed with the colony of laboratory Djungarian hamsters (Ph. sungorus) kept under 12L/12D photoperiod at a temperature of +22 ºC in standard cages (26 × 36 × 20 cm). Experimental animals (n = 36) were randomly divided into experimental and control groups: the experimental group included 10 males and 10 females; the control group included 8 males and 8 females.</p><p>During 80 days of experiment, hamsters in the experimental group were exposed to vapour from heating X-3 Yoghurt Pear liquid (PRIDE VAPE, Russia) containing glycerin and propylene glycol in a 70/30 ratio, nicotine at a dose of 3 mg/ml, and “Yogurt” and “Pear” flavouring agents. The vapour exposure consisted of inflowing cigarette vapour by means of a pump and filling with it the entire chamber two times with a 5-minute interval. After 10 minutes, the animals were removed from the containers. The procedure was performed daily, twice a day, with a 2-hour interval. Hamsters from the control group were delivered to the experimental room after removing the air with aerosol particles from the room, and then placed in the challenge chambers without exposure to ENDS vapour.</p><p>The experimental setup included a container for animal exposure to vapour. For this purpose, the plastic food containers of the dimensions 10 x 17 x 4 cm, and volume of 0.7 l, with tight-fitting lids were used. To optimize the process, two containers connected with 4 mm hoses (Boutte, Italy) were used simultaneously. A pump (Intex, China) with a volume of V~1.594 l was used to pump aerosol into the chambers.</p><p>To study the morphofunctional state of the lungs and main organs of detoxification, the lungs, kidneys, and livers of the animals from both groups were collected after decapitation and fixed in 10% neutral formalin. Tissue samples of these organs were dehydrated and clarified in isopropyl alcohol in compliance with the tissue processing protocol. The test specimens were embedded in paraffin blocks, and afterwards the series of 6-μm-thick slices were cut using a Slee Medical CUT 5062 rotary semiautomated microtome (SLEE Medical GmbH, Germany). These slices were mounted on glass slides using a 1:1 protein-glycerol mixture. The slides were stained with Böhmer’s hematoxylin and eosin. Collagen distribution was determined using the Mallory method [<xref ref-type="bibr" rid="cit34">34</xref>].</p><p>Histological preparations of the organs were examined under transmission light microscope Axio Imager M2 with AxioVision Z2 M2 image analysing module (Carl Zeiss, Germany). Images were taken using an AxioCam HR CCD camera with Zen Lite software (Carl Zeiss, Germany). All images contained a scale bar.</p><p>Statistical data were processed by calculating arithmetic means (x) and their errors (Sx). Differences in parameters between the experimental group compared to those in the control group were assessed using the Student’s t-test and were considered significant at p ≤ 0.05. All calculations were performed using commonly accepted formulas and Microsoft Excel 2010.</p><p>Results. The morphological pattern of the lung parenchyma of animals from the control group generally corresponded to the normal structure of this organ (Fig. 1 a, b, c). In the preparations stained with Böhmer’s hematoxylin and eosin, bronchi of various calibres were clearly visible (Fig. 1 a, c). In large bronchi, multilayered and columnar structure of epithelium was observed (Fig. 1 c). In the lumen, mucous secretion and weakly expressed desquamation of the epithelium were identified mainly at the site of transition of the terminal bronchioles into respiratory ones. Intralobular blood vessels were filled with blood plasma. The morphological pattern of the alveoli, which included capillary endothelial cells, type-1 and –2 alveolar cells, and macrophages, corresponded to the norm (Fig. 1 b, c) [35-36].</p><fig id="fig-1"><caption><p>Fig. 1. Lung specimen of a Djungarian hamster from the control group. Stained with Böhmer’s hematoxylin and eosin. Black arrow indicates bronchi; asterisk — columnar epithelium; black arrowhead — alveolar epithelium; light arrowhead — macrophages; oval — alveoli; square — epithelial desquamation</p></caption><graphic xlink:href="vetpatol-24-4-g001.jpeg"><uri content-type="original_file">https://cdn.elpub.ru/assets/journals/veterinary/2026/1/FdwOfEWKUoSuHej8ERbxpxpc4jsoK2QXjdRNVgvC.jpeg</uri></graphic></fig><p>In the examined lung tissue specimens of animals from the experimental group, changes affecting the lung parenchyma and interstitium were detected. In the specimens, alternating foci of atelectasis and emphysema were visible (Fig. 2a). Complexes of desquamated epithelial cells were visible in the lumen of the bronchi and bronchioles (Fig. 2a, b). The epithelium of the mucous membrane had lost its multilayered structure. At high magnification, the columnar epithelial cells were noticed to lose their cilia. In the lamina propria of the mucous membrane, signs of edema and swelling of the fibrous components of connective tissue were visible. Blood vessels of the lamina propria were excessively dilated, filled with plasma and blood cells. Among the latter, leukocytes were identified (Fig. 2c).</p><fig id="fig-2"><caption><p>Fig. 2. Lung specimen of a Djungarian hamster from the experimental group. Stained with Böhmer’s hematoxylin and eosin. The oval indicates an area of emphysema; the rectangle —atelectasis; the circle — epithelial desquamation; the black arrow — bronchial epithelium; the dotted arrow —leukocyte infiltration; the black arrowhead — plasma impregnation of the alveolar walls; the asterisk — edema of the lamina propria; the curly bracket — edema of the perivascular connective tissue. 2c: the black arrowhead indicates a type-2 alveolar cell; the asterisk — a type-1 alveolar cell</p></caption><graphic xlink:href="vetpatol-24-4-g002.jpeg"><uri content-type="original_file">https://cdn.elpub.ru/assets/journals/veterinary/2026/1/OebIzWJZJiV8iTeXTXk66hvqrkYu8xf0ienIuNQi.jpeg</uri></graphic></fig><p>The interalveolar septa and the walls of the alveolar sacs were thickened due to plasma impregnation and capillary congestion (Fig. 2a). Macrophages, segmented neutrophils, and lymphocytes were found in the alveolar lumens (Fig. 2c). A typical feature found in the lung specimens of animals from the experimental group was an excessive increase in the number of type-2 alveolar cells (Fig. 2c). Among type-1 epithelial cells, cells with pyknotic nuclei were often found. Capillaries and venules were congested. Perivascular connective tissue was loose and edematous. Endothelial cells of the alveolar capillaries were swollen. The nucleus was large, with a high content of heterochromatin, as a rule, and was bulged into the lumen of the capillaries (Fig. 2d).</p><p>A typical feature of lung tissue in animals from the experimental group was localization of homogeneous black substance among bronchial epithelial cells and in the interstitium of the alveolar sacs (Fig. 3a). A histochemical reaction for collagen according to Mallory method revealed intense staining of slices for this protein in the stroma at the periphery of segmental, intrasegmental, and intralobular bronchi, arteries, and veins of the lung. In the interstitium of the lung tissue, the reaction for collagen was moderate (Fig. 3b, c).</p><fig id="fig-3"><caption><p>Fig. 3. Lung specimen of a Djungarian hamster from the experimental group: a — staining with Böhmer’s hematoxylin and eosin; b, c — reaction for collagen according to Mallory method. The oval indicates the area of epithelial desquamation; the asterisk — positive reaction for collagen at the periphery of the segmental and intrasegmental bronchi; the black arrow — localization of homogeneous black substance</p></caption><graphic xlink:href="vetpatol-24-4-g003.jpeg"><uri content-type="original_file">https://cdn.elpub.ru/assets/journals/veterinary/2026/1/pLcN2Afqnqfy9sbbKu5Y15uiVX9JPceyvjiswRZZ.jpeg</uri></graphic></fig><p>When studying kidney specimens of hamsters from the experimental group, a statistically significant decrease in all studied parameters of the renal glomeruli was found compared to the control group, which indicates a decrease in the functional activity of the kidneys in animals exposed to vapour (Table 1).</p><table-wrap id="table-1"><caption><p>Table 1</p><p>Morphological features of the renal corpuscle structures</p><p>Note: * — differences between the parameters of the control and experimental groups were significant (p ≤ 0.05)</p></caption><table><tbody><tr><td>Renal corpuscle parameters</td><td>Control group</td><td>Experimental group</td></tr><tr><td>Renal corpuscle surface area, µm²</td><td>160.45 ± 1.24</td><td>117.95 ± 2.87*</td></tr><tr><td>Glomerulus size, μm²</td><td>131.97 ± 0.12</td><td>95.34 ± 0.17*</td></tr><tr><td>Urinary space, μm²</td><td>45.2 ± 0.21</td><td>34.58 ± 0.28*</td></tr></tbody></table></table-wrap><p>The glomerular vessels were excessively dilated, filled with plasma and blood cells. Endothelial and mesangial cells were swollen, erythrocytes had signs of sludge phenomenon (Fig. 4b, d). A typical pathomorphological feature of kidney specimens of animals from the experimental group was a high content of nephrothelial cells with signs of lethal damage in all parts of the nephron. As a rule, the cytoplasm in dying nephrocytes does not stain with hematoxylin and eosin, the nucleus is hyperchromatic, the nuclear membrane is not identifiable (Fig. 4a, с). In the lumen of the distal and proximal convoluted tubules, as well as in the cytoplasm of nephrocytes, a fine granular black substance was noticeable (Fig. 4c). This sign was especially pronounced in the lumen of the collecting ducts and among the epithelial cells of this part of the nephron (Fig. 4c).</p><fig id="fig-4"><caption><p>Fig. 4. Kidney specimen of a Djungarian hamster from the experimental group. Stained with Böhmer’s hematoxylin and eosin. The black arrowhead indicates nephrocytes with signs of lethal damage; the black arrow — fine granular black substance; the asterisk — erythrocytes with signs of sludge phenomenon</p></caption><graphic xlink:href="vetpatol-24-4-g004.jpeg"><uri content-type="original_file">https://cdn.elpub.ru/assets/journals/veterinary/2026/1/KIZ6OY7D6egXTajefGv16o2aw409KjBZtJCBDhnw.jpeg</uri></graphic></fig><p>At the light optical microscopy, hepatocytes of the centrilobular and periportal zones of the liver lobule of animals from the experimental group differed by tinctorial properties [<xref ref-type="bibr" rid="cit37">37</xref>]. The cytoplasm of light hepatocytes was intensely basophilic and filled with oxyphilic material (Fig. 5a, c). In liver specimens of hamsters from the experimental group, stained with hematoxylin and eosin, compared to the control group, the predominance of hepatocytes with pycnotic nuclei in the organ parenchyma was clearly visible (Fig. 5a, b). Upon detailed examination of the specimens, it became obvious that such cells were hepatocytes dying by apoptosis. Their distinctive features were pycnosis of the cells and margination of chromatin in the nucleus (Fig. 5c). The predominance of such cells in the centrilobular zone, responsible for detoxification, suggested that the liver of animals in the experimental group experienced a functional load that was beyond the physiological optimum, and its adaptive resources were not capable of providing an adequate response to the effect of toxic substances (Fig. 5c).</p><fig id="fig-5"><caption><p>Fig. 5. Liver specimen of a Djungarian hamster from the experimental group. Stained with Böhmer’s hematoxylin and eosin. The oval indicates the centrilobular zone of the liver lobule; the black arrow — hepatocytes with signs of apoptosis; the black arrowhead — hepatocytes with pyknotic nuclei</p></caption><graphic xlink:href="vetpatol-24-4-g005.jpeg"><uri content-type="original_file">https://cdn.elpub.ru/assets/journals/veterinary/2026/1/jeRcgSDc8LyRx9YyMrpcSoCg7HxDmhq0xU3t4pJD.jpeg</uri></graphic></fig><p>Discussion and Conclusion. The results of the study provide every reason to consider that the chosen design of hamster exposure to the vape aerosol results in structural and functional changes in the lungs, liver, and kidneys. Damage to the bronchial epithelium, alveolar epithelium, and microcirculatory endothelium was detected in the lungs. Light microscopy data do not allow us to identify damage to the structures of the air-blood barrier; however, the gross morphological changes detected in this compartment indicate a disruption in the structural and functional organization of the basal membranes of capillaries and epithelial cells. This is known to lead to impaired microcirculation in the lungs, increased permeability of pulmonary capillaries, and the development of pulmonary edema. This may explain the presence of interstitial and alveolar edema and distelectasis (alveolar collapse alternating with expansion) in the lung parenchyma, which develop with the participation of leukocytes and macrophages [38–39].</p><p>In accordance with complementarity principle, which postulates the unity of structure and function, the detected hemodynamic changes lead to the disruption of ventilation-perfusion relationships in lung tissue and to gas exchange disorder. The high level of type-2 alveolar cells in the tissue can be explained by an increase in their proliferative activity in response to damage to the alveolar epithelium by substances contained in the vape aerosol. In addition to their role in surfactant synthesis, type-2 alveolar cells are deemed to be ensuring the detoxification. The combination of the detected lung changes suggests the pathological features very similar to acute respiratory distress syndrome.</p><p>Excessive dilation of glomerular capillaries in the absence of hypercellularity and mesangial edema may be due to the direct impact of biologically active molecules on the capillary walls, leading to capillary damage and disruption of blood circulation. The presence of an unidentified homogeneous substance in the lumen of the proximal and distal sections of the nephron tubules and collecting ducts, suggests that this substance is transported through the glomerular basal membrane and enters the renal glomerulus from the general bloodstream. A decrease in the morphometric parameters of the structural components of the renal corpuscle in the kidney specimens of animals from the experimental group, compared to the control group, provides every reason to suspect a disruption of the renal filtration-reabsorption mechanism and the development of renal failure.</p><p>Despite the absence of the obvious signs of liver damage, the abundance of evolutionarily adapted to detoxification dark hepatocytes dying by apoptosis in the centrilobular zone of the liver lobule, indicates the involvement of toxic substances in this process, which enter the liver with the blood.</p></body><back><ref-list><title>References</title><ref id="cit1"><label>1</label><citation-alternatives><mixed-citation xml:lang="ru">Рудаков Н.А. История создания и продвижения электронных сигарет. Бизнес-образование в экономике знаний. 2019;1(12):76–82.</mixed-citation><mixed-citation xml:lang="en">Rudakov NA. 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