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    K Number
    DEN180047
    Device Name
    Aptima Mycoplasma genitalium Assay
    Manufacturer
    Hologic, Inc.
    Date Cleared
    2019-01-23

    (145 days)

    Product Code
    QEP
    Regulation Number
    866.3393
    Type
    Direct
    Panel
    Microbiology
    Reference & Predicate Devices
    N/A
    Why did this record match?
    Device Name :

    Aptima Mycoplasma genitalium Assay

    AI/MLSaMDIVD (In Vitro Diagnostic)TherapeuticDiagnosticis PCCP AuthorizedThirdpartyExpeditedreview
    Intended Use

    The Aptima Mycoplasma genitalium assay is an in vitro nucleic acid amplification test (NAAT) for the qualitative detection of ribosomal RNA (rRNA) from Mycoplasma genitalium on the fully automated Panther system. It is intended for use as an aid in the diagnosis of M. genitalium urogenital infections in male and female patients suspected of M. genitalium infection.

    The assay may be used to test the following specimens: clinician-collected and selfcollected vaginal swabs (in a clinical setting), clinician-collected endocervical swabs, female and male urine, clinician-collected male urethral swabs, and self-collected penile meatal swabs (in a clinical setting).

    For females, a vaginal swab is the preferred specimen type due to higher clinical sensitivity for detecting M. genitalium than other specimen types: however, female urine or clinician-collected endocervical swabs may be used as alternative specimens when vaginal swab specimens are not available. If female urine or clinician-collected endocervical swab specimens test negative, testing with a vaginal swab may be indicated, if M. genitalium infection is suspected.

    Device Description

    The Aptima Mycoplasma genitalium Assay is a nucleic acid amplification test to qualitatively detect ribosomal RNA from Mycoplasma genitalium. The assay is performed using the Panther System and includes three main processing steps: target capture, transcription-mediated amplification (TMA), and detection by nucleic acid hybridization. The Aptima Mycoplasma genitalium Assay oligonucleotides are designed to specifically capture, amplify, and detect a highly conserved region of Mycoplasma genitalium and the internal control (IC).

    The Aptima Mycoplasma genitalium Assay is provided as a 100-test kit. Following are the reagents and materials required to perform the assay on the Panther System:

    Aptima Mycoplasma genitalium Assay Kit

    • Amplification Reagent
    • Enzyme Reagent
    • Probe Reagent
    • Internal Control Reagent
    • Selection Reagent
    • Target Capture Reagent
    • Amplification Reconstitution Solution
    • Enzyme Reconstitution Solution
    • Probe Reconstitution Solution

    Aptima Mycoplasma genitalium Calibrators Kit

    • Negative Calibrator
    • Positive Calibrator

    Materials required but sold separately:

    • Aptima Assay Fluids Kit
    • Aptima Auto Detect Kit
    • Aptima Multitest Swab Specimen Collection Kit
    • Aptima Unisex Swab Specimen Collection Kit for Endocervical and Male Urethral Swab Specimens
    • Aptima Urine Specimen Collection Kit
    AI/ML Overview

    Aptima Mycoplasma genitalium Assay Study Summary

    This document describes the acceptance criteria and a prospective, multi-center clinical study conducted to establish the clinical performance characteristics of the Aptima Mycoplasma genitalium Assay.

    1. Acceptance Criteria and Reported Device Performance

    The acceptance criteria for this device are not explicitly stated as quantitative thresholds in the provided text (e.g., "sensitivity must be >X%"). Instead, the document presents detailed performance characteristics obtained from various studies, which are implicitly considered acceptable for the de novo classification. The key performance metrics are summarized below:

    Performance MetricAcceptance Criteria (Implicit)Reported Device Performance (Specificity from PIS Study)
    Sensitivity (Female Specimens)High sensitivity desired across specimen types, with vaginal swabs as preferred.Clinician-Collected Vaginal Swab: 92.0% (86.9-95.1%)
    Patient-Collected Vaginal Swab: 98.9% (95.9-99.7%)
    Endocervical Swab: 81.5% (75.1-86.6%)
    Female Urine: 77.8% (71.1-83.3%)
    Specificity (Female Specimens)High specificity desired across specimen types.Clinician-Collected Vaginal Swab: 98.0% (97.2-98.6%)
    Patient-Collected Vaginal Swab: 98.5% (97.7-99.0%)
    Endocervical Swab: 98.3% (97.5-98.8%)
    Female Urine: 99.0% (98.3-99.4%)
    Sensitivity (Male Specimens)High sensitivity desired across specimen types.Urethral Swab: 98.2% (94.8-99.4%)
    Penile Meatal Swab: 88.4% (82.6-92.5%)
    Male Urine: 90.9% (85.5-94.4%)
    Specificity (Male Specimens)High specificity desired across specimen types.Urethral Swab: 99.6% (99.1-99.8%)
    Penile Meatal Swab: 97.8% (96.9-98.5%)
    Male Urine: 99.4% (98.8-99.7%)
    Positive Percent Agreement (PPA) (Specimen-Specific)High PPA desired across specimen types.Clinician-Collected Vaginal Swab: 98.3% (95.2-99.4%)
    Patient-Collected Vaginal Swab: 98.9% (95.9-99.7%)
    Endocervical Swab: 97.0% (93.2-98.7%)
    Female Urine: 94.2% (89.4-96.9%)
    Urethral Swab: 98.2% (94.8-99.4%)
    Penile Meatal Swab: 95.3% (91.0-97.6%)
    Male Urine: 97.5% (93.9-99.0%)
    Negative Percent Agreement (NPA) (Specimen-Specific)High NPA desired across specimen types.Clinician-Collected Vaginal Swab: 98.9% (98.3-99.3%)
    Patient-Collected Vaginal Swab: 98.5% (97.7-99.0%)
    Endocervical Swab: 99.6% (99.1-99.8%)
    Female Urine: 99.4% (98.9-99.7%)
    Urethral Swab: 99.6% (99.1-99.8%)
    Penile Meatal Swab: 99.0% (98.3-99.4%)
    Male Urine: 99.9% (99.5-100%)
    Limit of Detection (LoD)LoD should be low, indicating high analytical sensitivity.Vaginal Swab: 0.04 - 0.10 GE/mL
    Female Urine: 0.04 - 0.12 GE/mL
    Penile Meatal Swab: 0.05 - 0.10 GE/mL
    Male Urine: 0.03 - 0.16 GE/mL
    Precision/ReproducibilityLow variability across different conditions (instruments, operators, lots, days, runs).%CV for S/CO: 5.58% - 16.21% (total variability for positive samples)
    % Agreement: 100% for all negative panel members, 100% for positive panel members in reproducibility study.
    Analytical Reactivity (Inclusivity)Ability to detect various Mycoplasma genitalium strains.9 Mycoplasma genitalium strains detected at ≥95% positivity, with most at low GE/mL concentrations.
    Analytical Specificity (Cross-reactivity)No false positives with common genitourinary flora and related microorganisms.No false positive test results with any of 56 tested microorganisms. In silico analysis showed no significant interactions.
    Microbial InterferenceNo, or minimal, interference from other microorganisms.No microbial interference observed, except with Mycoplasma pneumoniae (a limitation noted in the package insert).
    Interfering SubstancesNo interference from common gynecological/feminine hygiene products, bodily fluids.No interference observed with listed interfering substances at specified concentrations, except with mucus at 0.3% w/v (a limitation noted in the package insert).
    Carryover ContaminationNo carryover from high positive to negative samples.No carryover observed in checkerboard study.

    2. Sample Size and Data Provenance (Clinical Study)

    • Sample Size (Test Set):
      • Subjects: 3300 evaluable subjects (1737 women, 1563 men).
      • Specimens with Valid Aptima Results: 11,774.
      • Specimens with Valid PIS Results (used for Sensitivity/Specificity): 11,557.
      • Specimens with Specimen-Specific Composite Comparator Results (used for PPA/NPA): 11,665.
    • Data Provenance: Prospective, multi-center clinical study conducted at 21 US sites. Testing was performed at three sites.

    3. Number of Experts and Qualifications for Ground Truth (Clinical Study)

    The ground truth ("patient infected status" - PIS) was established using a "composite comparator algorithm comprised of three validated transcription mediated amplification (TMA) based assays for Mycoplasma genitalium." The document specifies that these comparator TMA assays were developed by Hologic (the applicant), as shown in section "O. Other Supportive Instrument Performance Characteristics Data Not Covered In The "Performance Characteristics" Section above: Comparator TMA Assays validation."

    Therefore, the ground truth was not established by human experts but by a composite of validated laboratory tests.

    4. Adjudication Method (Clinical Study)

    The PIS was determined using a composite comparator algorithm of three validated TMA assays.

    • Method: Two of the three comparator TMA assays had to be positive or negative to establish the infected or not-infected PIS, respectively.
    • Tie-breaker: The third TMA assay was run as a tie-breaker if the results of the first two TMA assays were discordant.

    5. Multi-Reader Multi-Case (MRMC) Comparative Effectiveness Study

    No, a multi-reader multi-case (MRMC) comparative effectiveness study was not explicitly described. This study evaluated the performance of a diagnostic device (the Aptima Mycoplasma genitalium Assay) against a composite reference standard (PIS), not the comparative effectiveness of human readers with or without AI assistance.

    6. Standalone Performance Study

    Yes, the study described is a standalone (algorithm only without human-in-the-loop performance) study. The Aptima Mycoplasma genitalium Assay is an in vitro diagnostic device (NAAT) whose performance characteristics (sensitivity, specificity, PPA, NPA) were directly evaluated against a composite reference standard. There is no indication of human interpretation or assistance being part of the device's output or the evaluation process.

    7. Type of Ground Truth Used (Clinical Study)

    The type of ground truth used was a composite comparator algorithm (laboratory-based), also referred to as "patient infected status (PIS)." This PIS was determined by the concordance of three validated transcription-mediated amplification (TMA) assays for Mycoplasma genitalium.

    8. Sample Size for the Training Set

    The document does not specify the sample size for a "training set." This is an in vitro diagnostic assay, and while it involves design and development, the primary clinical evaluation described is a prospective validation study. The analytical performance evaluations (e.g., LoD, inclusivity, cross-reactivity) involve testing various samples, but these are generally considered part of the verification and validation of the assay, not a distinct "training set" in the machine learning sense. The clinical study is a test set evaluation.

    9. How the Ground Truth for the Training Set Was Established

    As noted above, a distinct "training set" with independent ground truth establishment is not described in the context of this diagnostic assay's evaluation. The analytical studies establishing LoD, inclusivity, and specificity use characterized samples (e.g., spiked samples with known concentrations of M. genitalium or other microorganisms), which serve as their own form of "ground truth" for those specific analytical characteristics.

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