The GSTP1/MAPKs/BIM/SMAC modulatory actions of nitazoxanide: Bioinformatics and experimental evidence in subcutaneous solid Ehrlich carcinoma-inoculated mice

Imbaby, Samar; Elkholy, Shereen E.; Faisal, Salwa; Abdelmaogood, Asmaa K. K.; Mehana, AE; Mansour, Basma S.A.; El-moneam, Samar M. Abd; Elaidy, Samah M.

doi:10.1016/j.lfs.2023.121496

Cited by 15 publications

(3 citation statements)

References 88 publications

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“…The tissue sections were dewaxed using xylene (Beyotime, Shanghai, China) and rehydrated using gradient alcohol. Histological staining was performed using a haematoxylin and eosin (H&E) staining kit and a Masson’s staining kit (Solarbio, Beijing, China), followed by dehydration and transparency [ 25 , 26 ]. Neutral resin was used to seal the slices, which were observed under a light microscope (Tokyo, Japan).…”

Section: Methodsmentioning

confidence: 99%

miR-29b-1-5p exacerbates myocardial injury induced by sepsis in a mouse model by targeting TERF2

Jiang,

Xu,

Zeng

et al. 2024

ABBS

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Myocardial damage is a critical complication and a significant contributor to mortality in sepsis. MicroRNAs (miRNAs) have emerged as key players in sepsis pathogenesis. In this study, we explore the effect and mechanisms of miR-29b-1-5p on sepsis-induced myocardial damage. Sepsis-associated Gene Expression Omnibus datasets (GSE72380 and GSE29914) are examined for differential miRNAs. The mouse sepsis-induced cardiac injury was established by Lipopolysaccharide (LPS) or cecal ligation and puncture (CLP). LPS-treated HL-1 mouse cardiomyocytes simulate myocardial injury in vitro . miR-29b-1-5p is co-upregulated in both datasets and in cardiac tissue from sepsis mouse and HL-1 cell models. miR-29b-1-5p expression downregulation was achieved by antagomir transduction and confirmed by real-time quantitative reverse transcription PCR. Survival analysis and echocardiography examination show that miR-29b-1-5p inhibition improves mice survival cardiac function in LPS- and CLP-induced sepsis mice. Hematoxylin and eosin and Masson’s trichrome staining and Immunohistochemistry analysis of mouse myocardial α-smooth muscle actin show that miR-29b-1-5p inhibition reduces myocardial tissue injury and fibrosis. The inflammatory cytokines and cardiac troponin I (cTnI) levels in mouse serum and HL-1 cells are also decreased by miR-29b-1-5p inhibition, as revealed by enzyme-linked immunosorbent assay. The expressions of autophagy-lysosomal pathway-related and apoptosis-related proteins in the mouse cardiac tissues and HL-1 cells are evaluated by western blot analysis. The sepsis-induced activation of the autophagy-lysosomal pathway and apoptosis are also reversed by miR-29b-1-5p antagomir. MTT and flow cytometry measurement further confirm the protective role of miR-29b-1-5p antagomir in HL-1 cells by increasing cell viability and suppressing cell apoptosis. Metascape functionally enriches TargetScan-predicted miR-29b-1-5p target genes. TargetScan prediction and dual luciferase assay validate the targeting relationship between miR-29b-1-5p and telomeric repeat-binding factor 2 (TERF2). The expression and function of TERF2 in HL-1 cells and mice are also evaluated. MiR-29b-1-5p negatively regulates the target gene TERF2 . TERF2 knockdown partly restores miR-29b-1-5p antagomir function in LPS-stimulated HL-1 cells. In summary, miR-29b-1-5p targetedly inhibits TERF2, thereby enhancing sepsis-induced myocardial injury.

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Section: Methodsmentioning

confidence: 99%

miR-29b-1-5p exacerbates myocardial injury induced by sepsis in a mouse model by targeting TERF2

Jiang,

Xu,

Zeng

et al. 2024

ABBS

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“…The DNeasy extraction kit (Qiagen, Hilden, Germany) was used to extract genomic DNA as per the manufacturer's manual. A Nanodrop ND-1000 spectrophotometer (NanoDrop Technologies, Wilmington, USA) was utilized to determine the quality and quantity of the extracted DNA [14]. All MRSA isolates were screened for the presence of efflux pump genes norA, norB and norC using their specific primers sequences (Table 1).…”

Section: Dna Extraction and Detection Of Efflux Pump Genes Using The ...mentioning

confidence: 99%

Expression of norA, norB and norC efflux pump genes mediating fluoroquinolones resistance in MRSA isolates

Hamady,

Abd El-Fadeal,

Imbaby

et al. 2024

J Infect Dev Ctries

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Introduction: Although fluoroquinolones are used to treat methicillin-resistant Staphylococcus aureus (MRSA)-induced infections, acquisition of antibiotic resistance by bacteria has impaired their clinical relevance. We aimed to evaluate the frequency of norA, norB, and norC efflux pump genes-mediating fluoroquinolones resistance and measure their expression levels in MRSA isolates. Methodology: 126 S. aureus isolates were collected from different clinical samples of adult hospitalized patients and identified by conventional microbiological methods. MRSA was diagnosed by cefoxitin disc diffusion method and minimum inhibitory concentration (MIC) of ciprofloxacin by broth microdilution method. The expression levels of efflux pump genes were measured by quantitative real-time polymerase chain reaction (qRT-PCR). Results: 80 (63.5%) MRSA isolates were identified and showed high level of resistance to erythromycin (80%), gentamicin (75%), clindamycin (65%) and ciprofloxacin (60 %). norA, norB and norC were detected in 75%, 35% and 55% of the MRSA isolates respectively. norC was the most commonly overexpressed gene measured by qRT-PCR, occurring in 40% of MRSA isolates, followed by norA (35%) and norB (30%). The expression of these genes was significantly higher in ciprofloxacin-resistant than quantitative real-time PCR ciprofloxacin-sensitive MRSA isolates. Conclusions: This study showed high prevalence and overexpression of efflux pump genes among MRSA isolates which indicates the significant role of these genes in the development of multidrug resistance against antibiotics including fluoroquinolones.

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“…Известны данные о том, что экспериментальные животные с солидной формой карциномы Эриха живут дольше, чем с АКЭ. Число хромосом в клетках модального класса 44-46, при этом в клетках обнаруживаются маркерные хромосомы, типичные для АКЭ [5].…”

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The Evaluation of Hematological Blood Parameters in Laboratory Mice Tumor Ehrlich’s Adenocarcinoma Carrier

Соболева,

Тихонович,

Жогаль

et al. 2023

Лабораторная Диагностика. Восточная Европа

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Введение. Разработка новых подходов к лечению онкологических заболеваний с использованием мышей – опухоленосителей аденокарциномы Эрлиха актуальна, поскольку данный аспект исследования позволяет получить адекватные, воспроизводимые результаты, имеющие перспективы применения в клинической практике. Однако анализ сведений из источников доступной научной литературы показал недостаточную изученность изменения гематологических показателей крови у лабораторных мышей-опухоленосителей. Цель. Оценка особенностей изменения морфологической картины крови мышей – опухоленосителей карциномы Эрлиха при разных, удовлетворяющих требованиям проведения эксперимента, ее биологических моделях. Материалы и методы. Исследование осуществлено на самках аутбредных мышей ICR и самцах инбредных мышей линии Af 2–3-месячного возраста, массой 20,0±2,0 г. Экспериментальные группы были сформированы следующим образом: группа 1 – моделирование АКЭ проводили внутрибрюшинным введением клеток аденокарциномы Эрлиха (в/б) самкам аутбредных мышей ICR (n=20); группа 2 – моделирование СКЭ проводили подкожным введением клеток аденокарциномы Эрлиха (п/к) самкам аутбредных мышей ICR (n=20); группа 3 – моделирование СКЭ проводилось подкожным введением клеток аденокарциномы Эрлиха (п/к) самцам инбредных мышей Af (n=20). Для перевивки опухоли был использован гипердиплоидный штамм аденокарциномы Эрлиха. Кровь забирали из лицевой вены мышей. Гематологические показатели определяли на автоматическом анализаторе URIT VET3000 Plus. Для подсчета лейкоцитарной формулы окрашенные по Романовскому – Гимзе мазки крови просматривали на световом микроскопе LEICA DM2500. Статистическую обработку данных проводили с использованием t-критерия Вилкоксона для зависимых выборок. Результаты между независимыми выборками анализировали с помощью критерия Манна – Уитни. Различия считали достоверными при р<0,05. Результаты. В исследовании установлены гематологические критерии развития опухолевого процесса в период 14 суток после ксенотрансплантации клеток аденокарциномы Эрлиха в объеме 0,2 мл в количестве 2×106 морфологических единиц. В эксперименте на животных созданы модели асцитной карциномы Эрлиха (АКЭ) и ее солидной формы (СКЭ) у самок мышей линии ICR и самцов мышей линии Af. Кровь забирали из лицевой вены мышей два раза: первый раз до прививки опухоли и второй раз на 14-е сутки развития опухолевого процесса. Выделены зависимые и независимые ни от вида, ни от пола, ни от способа инокуляции клеток аденокарциномы Эрлиха изменения параметров морфологической картины крови экспериментальных животных. Заключение. Ксенотрансплантация аденокарциномы Эрлиха мышам к 14-м суткам сопровождается следующими изменениями: в распределении эритроцитов по объему; среднем объеме тромбоцитов, распределении тромбоцитов по объему, количестве лимфоцитов, нейтрофилов, эозинофилов и не оказывает влияния на уровень базофилов крови. Количественные показатели крови мышей-опухоленосителей перспективны для обоснования выбора тест-систем и сопоставления эффективности потенциальных противоопухолевых субстанций, способных повлиять на систему крови. Introduction. The study of new approaches in the treatment of oncological diseases using Ehrlich adenocarcinoma mice is relevant and allows obtaining adequate, reproducible results that have prospects for application in clinical practice. However, the analysis of the sources of scientific literature showed a poor study of hematological blood parameters in laboratory mice-tumor carriers. Purpose. Evaluation of the peculiarities of changes in the morphological picture of blood of Ehrlich carcinoma tumor-bearing mice under different, satisfying the requirements of the experiment, its biological models. Materials and methods. The work was performed on female outbred ICR mice and male inbred Af mice aged 2–3 months, weighing 20.0±2.0 g. The experimental groups were formed as follows: group 1 – EAC modeling was performed by intraperitoneal injection of Ehrlich adenocarcinoma cells to female outbred ICR mice (n=20); group 2 – ESC modeling was performed by subcutaneous injection of Ehrlich adenocarcinoma cells to female outbred ICR mice (n=20); group 3 – ESC modeling was performed by subcutaneous injection of Ehrlich adenocarcinoma cells to male inbred Af mice (n=20). A hyperdiploid strain of Ehrlich’s adenocarcinoma was used for tumor transplantation. Blood was taken from the facial vein of mice. Hematological parameters were determined on an automatic analyzer URIT VET3000 Plus. To calculate the leukocyte count, Romanovsky – Giemsa- stained blood smears were examined using a LEICA DM2500 light microscope. Statistical processing was performed using the Wilcoxon t-test for dependent samples. The results between independent samples were analyzed using the Mann – Whitney test. Differences were considered significant at p<0.05. Results. Hematological criteria of the tumor process development in the period of 14 days after xenotransplantation of 0,2 ml Erlich adenocarcinoma cells in the amount of 2×106 morphological units were established in the research. We modeled Ehrlich ascites carcinoma (EAC) and its solid form (ESC) in female ICR mice and male ICR mice. Blood was collected from the facial vein of mice twice: the first time before tumor inoculation and the second time on the 14th day of tumor development. We distinguished the changes of the internal environment parameters which were dependent on neither species, nor sex, nor the way of Ehrlich adenocarcinoma cell inoculation. Conclusion. Xenotransplantation of adenocarcinoma of Ehrlich into mice by 14 days is accompanied by the following changes in: red blood cell volume distribution; average volume of platelets, distribution of platelets by volume, the number of lymphocytes, neutrophils, eosinophils, and has no effect on the level of blood basophils. Quantitative blood indicators of tumor-bearing mice are promising for justifying the choice of test system and the effectiveness of the strategy for the effectiveness of antitumor substances capable of indicators in the blood system.

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The GSTP1/MAPKs/BIM/SMAC modulatory actions of nitazoxanide: Bioinformatics and experimental evidence in subcutaneous solid Ehrlich carcinoma-inoculated mice

Cited by 15 publications

References 88 publications

miR-29b-1-5p exacerbates myocardial injury induced by sepsis in a mouse model by targeting TERF2

miR-29b-1-5p exacerbates myocardial injury induced by sepsis in a mouse model by targeting TERF2

Expression of norA, norB and norC efflux pump genes mediating fluoroquinolones resistance in MRSA isolates

The Evaluation of Hematological Blood Parameters in Laboratory Mice Tumor Ehrlich’s Adenocarcinoma Carrier

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