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Rapid Detection and Quantification of Viable Cells of Pectobacterium brasiliense Using Propidium Monoazide Combined with Real-Time PCR.


ABSTRACT: Pectobacterium brasiliense (Pbr) has caused significant economic losses in major vegetable production areas in Northern China by causing bacterial soft rot in cash crops such as potatoes and cucumbers. This study aimed to establish a PMA-qPCR detection method for Pbr by screening specific and sensitive primers based on the glu gene and the conserved region of the 23S rRNA gene. Based on the optimized PMA pretreatment conditions, a standard curve was designed and constructed for PMA-qPCR detection (y = -3.391x + 36.28; R2 = 0.99). The amplification efficiency reached 97%, and the lowest detection limit of viable cells was approximately 2 × 102 CFU·mL-1. The feasibility of the PMA-qPCR method was confirmed through a manually simulated viable/dead cell assay under various concentrations. The analysis of potato tubers and cucumber seeds revealed that nine naturally collected seed samples contained a range from 102 to 104 CFU·g-1 viable Pbr bacteria. Furthermore, the system effectively identified changes in the number of pathogenic bacteria in cucumber and potato leaves affected by soft rot throughout the disease period. Overall, the detection and prevention of bacterial soft rot caused by Pbr is crucial.

SUBMITTER: Li J 

PROVIDER: S-EPMC10673545 | biostudies-literature | 2023 Nov

REPOSITORIES: biostudies-literature

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Rapid Detection and Quantification of Viable Cells of <i>Pectobacterium brasiliense</i> Using Propidium Monoazide Combined with Real-Time PCR.

Li Junhui J   Chen Ruxing R   Yang Ruwei R   Wei Xinchen X   Xie Hua H   Shi Yanxia Y   Xie Xuewen X   Chai Ali A   Fan Tengfei T   Li Baoju B   Li Lei L  

Microorganisms 20231119 11


<i>Pectobacterium brasiliense</i> (<i>Pbr</i>) has caused significant economic losses in major vegetable production areas in Northern China by causing bacterial soft rot in cash crops such as potatoes and cucumbers. This study aimed to establish a PMA-qPCR detection method for <i>Pbr</i> by screening specific and sensitive primers based on the <i>glu</i> gene and the conserved region of the 23S rRNA gene. Based on the optimized PMA pretreatment conditions, a standard curve was designed and const  ...[more]

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