Search Results

1.Emerging Pathogenetic Mechanisms of Pulmonary Arterial Hypertension: Nitric Oxide and More.

Young Dae KIM

Korean Circulation Journal 2011;41(2):58-60

2.Emerging Pathogenetic Mechanisms of Pulmonary Arterial Hypertension: Nitric Oxide and More.

Young Dae KIM

Korean Circulation Journal 2011;41(2):58-60

3.Nitric Oxide: The Pathophysiological Roles and Clinical Implications in Circulatory System.

Kwang Youn LEE

Yeungnam University Journal of Medicine 1996;13(2):159-172

4.Endogenous nitric oxide mediates the renal response to amino acid infusion.

Ki Chul CHOI ; Suhn Hong UHM ; Seung Min PARK ; Jong Eun LEE ; Young Joon KANG

Korean Journal of Nephrology 1993;12(4):505-511

5.Optimization of cell density and LPS concentration for the evaluation of nitric oxide production on BV-2 in a Griess assay

Nasim Karimi Hosseini ; Shinsmon Jose ; Sharmili Vidyadaran ; Syafinaz Amin Nordin

Malaysian Journal of Medicine and Health Sciences 2014;10(2):1-8

Introduction: Production of nitric oxide (NO) is one of the main responses elicited by a variety of immune cells such as macrophages (e.g. microglia, resident macrophages of brain), during inflammation. Evaluation of NO levels in the inflammatory milieu is considered important to the understanding of the intensity of an immune response; and has been performed using different methods including the Griess assay. To assay NO in culture, an appropriate number of cells are stimulated into an inflammatory phenotype. Common stimuli include lipopolysaccharide (LPS), IFN-γ and TNF-α. However, overt stimulation could cause cell cytotoxicity therefore an ideal concentration of LPS should be used. Objective: To set-up a model of BV-2 cell activation that allows the assay of detectable levels of NO. Optimization of BV-2 microglia cell density and LPS concentrations after stimulation by bacterial lipopolysaccharide (LPS) for the Griess assay is demonstrated in this study. Methods: BV-2 microglia were cultured at different cell densities, and treated with LPS at three concentrations (1, 5, 10 µg/ml). NO production in culture supernatants were then measured at 18, 24, 48 and 72 hours. Moreover, methyl tetrazolium assay (MTT) was also performed to ensure that NO measurement is performed at no-cytotoxic concentrations of LPS. Results and Conclusions: NO production follows a temporal pattern. The density of 25000 cells/ well was the ideal seeding density for NO evaluation in BV-2 cells. BV-2 stimulation by LPS is dose dependent, and NO levels are increased proportional to the LPS concentration up to 1.0µg/ml, whereas the higher LPS concentrations are associated with decreased cell viability may be caused by the high toxic levels of LPS or NO. Although Griess assay has been commonly used by the scientists, however, optimization of its parameters on BV-2 cells will be useful for the experiments which will be performed on this particular cell line. The optimized pattern of Griess assay on BV-2 cells was achieved in this study, hence easier and more practical for the future scientists to perform Griess assay on BV-2 cells.
Nitric Oxide

6.Biological Role of Nitric Oxide.

Hyeyoung KIM

The Korean Journal of Critical Care Medicine 1998;13(2):139-146

7.Endothelium-Derived Nitric Oxide

Jang Sang PARK

Journal of the Korean Society for Vascular Surgery 1998;14(2):179-193

8.Role of nitric oxide and distribution of nitric oxide synthase in the gustatory system.

Young Jae KIM ; Won Jae KIM ; Sun Youl RYU

Journal of the Korean Association of Oral and Maxillofacial Surgeons 2000;26(3):262-269

9.Isolation of Constituents with Nitric Oxide Synthase Inhibition Activity from Phryma leptostachya var. asiatica

Donghwa KIM ; Sang Kook LEE ; Kyoung Sik PARK ; Na Yun KWON ; Hee Juhn PARK

Natural Product Sciences 2019;25(1):34-37

10.Clinical application of fractional exhaled nitric oxide in pediatric allergic rhinitis.

Doo Hee HAN

Allergy, Asthma & Respiratory Disease 2015;3(6):385-386