Anticandidal and In vitro Anti-Proliferative Activity of Sonochemically synthesized Indium Tin Oxide Nanoparticles

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作者
Suriya Rehman
Sarah Mousa Asiri
Firdos Alam Khan
B. Rabindran Jermy
Vijaya Ravinayagam
Zainab Alsalem
Reem Al Jindan
Ahsanulhaq Qurashi
机构
[1] Department of Epidemic Diseases Research,
[2] Institute for Research & Medical Consultations,undefined
[3] (IRMC),undefined
[4] Imam Abdulrahman Bin Faisal University,undefined
[5] Department of Biophysics,undefined
[6] Institute for Research & Medical Consultations,undefined
[7] (IRMC),undefined
[8] Imam Abdulrahman Bin Faisal University,undefined
[9] Department of Stem Cell Research,undefined
[10] Institute for Research & Medical Consultations,undefined
[11] (IRMC),undefined
[12] Imam Abdulrahman Bin Faisal University,undefined
[13] Department of Nano-Medicine Research,undefined
[14] Institute for Research & Medical Consultations,undefined
[15] (IRMC),undefined
[16] Imam Abdulrahman Bin Faisal University,undefined
[17] Department of Microbiology,undefined
[18] College of medicine,undefined
[19] Imam Abdulrahman Bin Faisal University,undefined
[20] Center of excellence in nanotechnology,undefined
[21] King Fahd University of petroleum and Minerals Dhahran 31261 Saudi Arabia and Department of Chemistry,undefined
[22] Khalifa University of Science and Technology,undefined
[23] Main Campus,undefined
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The present work demonstrates the synthesis, characterization and biological activities of different concentrations of tin doped indium oxide nanoparticles (Sn doped In2O3 NPs), i.e., (Sn/In = 5%, 10% and 15%). We have synthesized different size (38.11 nm, 18.46 nm and 10.21 nm) of Sn doped In2O3 NPs. by using an ultra-sonication process. The Sn doped In2O3 NPs were characterized by by x-ray diffraction (XRD), scanning electron microscopy (SEM), and transmission electron microscopy (TEM) which confirmed the successful doping of tin (Sn) with Indium oxide (In2O3). Anticandidal activity was performed by standard agar dilution method using Candida albicans for the study. The minimum inhibitory/fungicidal concentration (MIC/MFC) values recorded were, 8 & >8 mg/ml for pure In2O3 NPs, 4 & 8 mg/ml for 5%, 2 & 8 mg/ml for 10%, whereas 1 & >4 mg/ml for 15% Sn doped In2O3 NPs, respectively. The topographical alteration caused by Sn doped In2O3 NPs on Candida cells, was clearly observed by SEM examination. A significant enhancement in anticandidal activity was seen, when Candida cells were exposed to (Sn/In = 5%, 10% and 15%). Moreover, we have also evaluated the impact of Sn-In2O3 NPs on human colorectal carcinoma cells (HCT-116). The results demonstrated that Sn-In2O3 NPs (Sn/In = 5%, 10% and 15%), caused dose dependent decrease in the cancer cell viability as the low dosage (2.0 mg/mL) showed 62.11% cell viability, while 4.0, 8.0, 16.0, 32.0 mg/mL dosages showed 20.45%, 18.25%, 16.58%, and 15.58% cell viability. In addition, the treatment of Sn-In2O3 NPs also showed significant cellular and anatomical changes in cancer cells as examined by microscopes. We have also examined the impact of Sn-In2O3 NPs (5%, 10%, 15%) on normal cells (HEK-293) and the results demonstrate that Sn-In2O3 NPs did not reduce the cell viability of normal cells.
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