Detecting and quantifying Veillonella by real-time quantitative PCR and droplet digital PCR

Ding, Zanbo; Cui, Jinghua; Zhang, Qun; Feng, Junxia; Du, Bing; Xue, Guanhua; Yan, Chao; Gan, Lin; Fan, Zheng; Feng, Yanling; Zhao, Hanqing; Xu, Ziying; Yu, Zihui; Fu, Tongtong; Zhang, Rui; Cui, Xiaohu; Tian, Ziyan; Chen, Jinfeng; Chen, Yujie; Li, Zhoufei; Zhong, Xuemei; Lin, Yanbing; Yuan, Jing

doi:10.1007/s00253-023-12861-1

Cited by 2 publications

(1 citation statement)

References 46 publications

(26 reference statements)

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“…In recent years, dPCR methods have been described for the specific diagnosis of numerous microorganisms. Thus, methods for the specific diagnosis of Veillonella have been described [42]. In this study, the sensitivity of dPCR was 11.3 copies/µL, while the sensitivity of qPCR was 100 copies/µL, though qPCR had a wider detection range than ddPCR.…”

Section: Bacteriology Applicationsmentioning

confidence: 68%

Present and Future Applications of Digital PCR in Infectious Diseases Diagnosis

Sancha Dominguez,

Cotos Suárez,

Sánchez Ledesma

et al. 2024

Diagnostics

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Infectious diseases account for about 3 million deaths per year. The advent of molecular techniques has led to an enormous improvement in their diagnosis, both in terms of sensitivity and specificity and in terms of the speed with which a clinically useful result can be obtained. Digital PCR, or 3rd generation PCR, is based on a series of technical modifications that result in more sensitive techniques, more resistant to the action of inhibitors and capable of direct quantification without the need for standard curves. This review presents the main applications that have been developed for the diagnosis of viral, bacterial, and parasitic infections and the potential prospects for the clinical use of this technology.

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Section: Bacteriology Applicationsmentioning

confidence: 68%

Present and Future Applications of Digital PCR in Infectious Diseases Diagnosis

Sancha Dominguez,

Cotos Suárez,

Sánchez Ledesma

et al. 2024

Diagnostics

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Dysregulation of lncRNA MALAT1 Contributes to Lung Cancer in African Americans by modulating the tumor immune microenvironment

Li,

Dhilipkannah,

Holden

et al. 2024

Preprint

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African American (AA) populations present with notably higher incidence and mortality rates from lung cancer in comparison to other racial groups. Here, we elucidate the contribution of long non-coding RNAs (lncRNAs) in the racial disparities and their potential clinical applications in both diagnosis and therapeutic strategies. AA patients had elevated plasma levels of MALAT1 and PVT1 compared with cancer-free smokers. Incorporating these lncRNAs as plasma biomarkers, along with smoking history, achieved 81% accuracy in diagnosis of lung cancer in AA patients. We observed a rise in MALAT1 expression, correlating with increased levels of monocyte chemoattractant protein-1 (MCP-1) and CD68, CD163, CD206, indicative of tumor-associated macrophages in lung tumors of AA patients. Forced MALAT1 expression led to enhanced growth and invasiveness of lung cancer cells, both in vitro and in vivo, accompanied by elevated levels of MCP-1, CD68, CD163, CD206, and KI67. Mechanistically, MALAT1 acted as a competing endogenous RNA to directly interact with miR-206, subsequently affecting MCP-1 expression and macrophage activity, and enhanced the tumorigenesis. Targeting MALAT1 significantly reduced tumor sizes in animal models. Therefore, dysregulated MALAT1 contributes to lung cancer disparities in AAs by modulating the tumor immune microenvironment through its interaction with miR-206, thereby presenting novel diagnostic and therapeutic targets.

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Detecting and quantifying Veillonella by real-time quantitative PCR and droplet digital PCR

Cited by 2 publications

References 46 publications

Present and Future Applications of Digital PCR in Infectious Diseases Diagnosis

Present and Future Applications of Digital PCR in Infectious Diseases Diagnosis

Dysregulation of lncRNA MALAT1 Contributes to Lung Cancer in African Americans by modulating the tumor immune microenvironment

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