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Application of Bacterial DNA Quantitative Detection in Diagnosis of SBP in Cirrhosis: A Multi Center Diagnostic Experiment

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Capital Medical University

Status

Invitation-only

Conditions

Cirrhosis
Bacterial Infections
Ascites

Treatments

Diagnostic Test: Bacterial DNA Levels in Ascites

Study type

Observational

Funder types

Other

Identifiers

NCT06995846
LL-2024-034-K

Details and patient eligibility

About

Background and Significance:

Spontaneous bacterial peritonitis (SBP) is a common and life-threatening complication in patients with liver cirrhosis, characterized by high incidence and mortality. The current diagnostic standard relies on ascitic fluid polymorphonuclear leukocyte (PMN) count ≥250 cells/μL. However, this threshold is associated with high rates of missed diagnoses, poor correlation with clinical symptoms, and delays in pathogen identification due to the low sensitivity and prolonged time of traditional ascitic fluid culture.

With the development of molecular diagnostics, bacterial DNA (bactDNA) detection-especially through droplet digital PCR (ddPCR)-has emerged as a promising technique due to its high sensitivity, absolute quantification capability, and robustness. This study aims to evaluate the diagnostic value and accuracy of ddPCR-based quantification of bacterial DNA in ascitic fluid for SBP, providing a novel and objective diagnostic tool to improve early and accurate detection and to inform targeted antimicrobial therapy.

Objectives:

To assess the diagnostic accuracy (sensitivity, specificity, predictive values) of ddPCR-based quantification of total bacterial DNA in ascitic fluid for SBP.

To evaluate the diagnostic performance of the ratio of Gram-positive to Gram-negative bacterial DNA (G+/G-) in predicting SBP.

To explore the potential of ddPCR-based bacterial DNA quantification as a complementary or alternative method to conventional PMN-based diagnostic criteria.

Study Design and Methods:

This is a prospective diagnostic study involving 700 patients with liver cirrhosis and ascites. Ascitic fluid samples will be analyzed using ddPCR to quantify bacterial DNA levels. These results will be compared with traditional diagnostic criteria, including PMN counts and expert panel assessments based on clinical symptoms and laboratory findings. Statistical analyses will include correlation analysis, ROC curve analysis, and consistency testing.

Expected Outcomes:

The study aims to establish the clinical efficacy of ddPCR-based quantification of bacterial DNA in ascitic fluid as a novel diagnostic marker for SBP. This method is expected to be particularly useful in atypical cases where PMN counts are <250/μL and may help guide preliminary antibiotic selection based on the proportion of Gram-positive and Gram-negative bacteria, thereby reducing empirical treatment failures and antibiotic resistance.

Enrollment

700 estimated patients

Sex

All

Ages

18+ years old

Volunteers

No Healthy Volunteers

Inclusion criteria

  • Age ≥ 18 years, no restriction on gender.
  • Diagnosis of liver cirrhosis based on imaging, biochemical, or hematological evidence of impaired hepatic synthetic function or portal hypertension, or histologically confirmed cirrhosis, regardless of etiology.
  • Diagnosis of ascites according to the 2023 Chinese Clinical Guidelines for the Diagnosis and Treatment of Cirrhotic Ascites and Related Complications.

Exclusion criteria

  • Patients with confirmed infections in other tissues or organs.
  • Ascites caused by non-hepatic etiologies, such as renal or cardiac ascites.
  • Pregnant individuals, intravenous drug users, or HIV-infected individuals.
  • Patients with uncontrolled hepatocellular carcinoma or other systemic malignancies.
  • Patients who have previously undergone organ transplantation.
  • Patients currently receiving glucocorticoids or other immunosuppressive therapies.

Trial design

700 participants in 1 patient group

Cirrhotic Patients with Ascites
Description:
Cirrhotic Patients with Ascites
Treatment:
Diagnostic Test: Bacterial DNA Levels in Ascites

Trial contacts and locations

1

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Data sourced from clinicaltrials.gov

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