Syphilis Kit 510k (Quantitative Test Kit) 510k and IVDR Process
A quantitative syphilis test kit is an in vitro diagnostic (IVD) assay designed to measure the concentration or titer of nontreponemal antibodies (reagin antibodies) generated during Treponema pallidum infection. These assays yield quantitative results expressed as numerical titers (e.g., 1:8, 1:32) that reflect antibody levels associated with disease activity. Quantitative syphilis assays are primarily used to monitor treatment response, assess disease progression, and detect reinfection, providing objective information on changes in antibody titers over time. Unlike treponemal qualitative assays that only determine the presence or absence of antibodies, quantitative nontreponemal assays enable serial titer comparison, supporting clinical decision-making in ongoing patient management.
COMPONENTS OF A QUANTITATIVE SYPHILIS TEST KIT
1. Antigen / Solid Phase – Cardiolipin–lecithin–cholesterol antigen complex (may include carbon or latex particles).
2.Calibrators / Titer Standards – Serially diluted reference sera with assigned titers for generating calibration curves.
3.Positive Control – Reactive control serum to verify assay performance.
4.Negative Control – Non-reactive control serum to confirm specificity and rule out false positives.
5.Internal / Procedural Control – Built-in system suitability or instrument control to validate each run.
6.Assay Buffers and Solutions – Sample diluent, reaction buffer, wash solutions, and stabilizers.
7.Detection Reagent / Signal Generation System – Carbon/latex particles or optical/chemiluminescent detection reagents for quantitation.
8.Test Platform / Consumables – Microplates, cuvettes, reaction tubes, or analyzer-specific cartridges required for quantitative reading.
Syphilis Quantitative Test Kit - Principle of Operation
Intended Use, Classification and Regulatory Information
The intended use is “Clinical diagnostic use (e.g., measuring reagin antibody titers in patient serum or plasma to aid in the assessment of syphilis disease activity, evaluation of treatment response, and identification of reinfection).” Quantitative nontreponemal syphilis assays—such as automated or manual RPR/VDRL titer-based methods—are regulated by the FDA as Class II devices. Submission is through the 510(k) premarket notification pathway, where manufacturers must demonstrate substantial equivalence to a legally marketed predicate, including evidence of analytical performance, calibration traceability, and reproducibility across clinically relevant titer ranges.
| Test Category | Intended Use | FDA Product Code | 21 CFR Regulation | Device Class | Submission Pathway |
| Non-Treponemal Quantitative | Qualitative and semi-quantitative detection of nontreponemal (reagin) antibodies to Treponema pallidum in human serum or plasma. | GMQ | 21 CFR 866.3820 | Class II | 510(k) |
For a detailed proposal with a Statement of Work, please complete the Request for Quote (RFQ) form provided separately for FDA 510(k) and IVDR CE Marking for Syphilis Kit 510k (Quantitative Kit)
Performance Evaluation
Scientific Validation
Scientific validation is an essential early phase carried out before full analytical validation. It establishes that the assay concept, design elements, and core reagents function as intended and are appropriate for further development. Regulatory bodies such as the FDA and CE expect preliminary evidence showing that the test demonstrates baseline specificity, sensitivity, and reliability before proceeding to extensive analytical studies. This stage confirms that the assay can consistently detect the target analyte in the intended specimen type under expected conditions, minimizing the risk of assay failure during formal validation. Scientific validation also strengthens regulatory submissions by providing foundational performance data and supporting compliance with quality system requirements (e.g., FDA 21 CFR Part 820, ISO 13485). Overall, it is a recommended and critical phase that helps ensure the test is on the right path to meeting safety and effectiveness standards prior to detailed analytical and clinical validation.
Analytical Validation
FDA requires comprehensive analytical evidence demonstrating that a quantitative syphilis assay accurately measures reagin antibody titers and supports its intended clinical use for disease monitoring, treatment evaluation, and reinfection assessment.
Reference Standards
• CLSI: EP05, EP06, EP17, MM03, EP09
• ISO: 13485, 15189
• WHO: International reference materials or panels for nontreponemal antibody titers, where available, to support calibration and traceability
Test parameters and acceptance criteria
| S.NO | Parameter | Purpose / Description | Typical Acceptance Criteria |
| 1 | Linearity / Dynamic Range | Demonstrate proportional response across serial dilutions. | R² ≥ 0.98; slope 0.9–1.1 |
| 2 | Accuracy / Method Comparison | Bias within ±1 dilution or ±15 % | Correlation vs. predicate qualitative titers ≥ 95 % |
| 3 | Precision / Reproducibility | Repeatability across sites, days, and operators. | CV ≤10% or ≥95% titer concordance |
| 4 | Analytical Sensitivity (LoQ) | Lowest measurable titer and quantitation limit. | “CV ≤ 20% & bias ≤ ±10% |
| 5 | Matrix Equivalence | Serum vs plasma comparison. | ≥95% correlation |
| 6 | Interference / Specificity | Evaluate impact of hemolysis, lipemia, bilirubin, or cross-reactivity. | ≤5% deviation or ≤2% false reactivity |
| 7 | Stability | Assess reagent performance over shelf life. | Within ±10% of baseline |
Pre-Analytical and Analytical Workflow
Testing Factors Overview
| Analyte / Target | Intended Use | Method | Sample Type | Acceptance Criteria |
| Reagin antibody (quantitative) | Determine antibody titer to monitor disease activity or treatment response | Manual or automated flocculation (RPR/VDRL) | Serum or plasma | Linearity R² ≥ 0.98; PPA/NPA ≥95% |
| Reagin antibody (semi-quantitative) | Establish endpoint titer by serial dilution | Card or slide-based test | Serum or plasma | ±1 dilution agreement ≥95% |
| Automated quantitative assays | Continuous optical or algorithmic quantification | Nephelometric or photometric system | Serum or plasma | Correlation R² ≥ 0.98; CV ≤10% |
| Calibrators / Standards | Generate regression or titer conversion curve | Instrument-based calibration | Internal reference | ≤10% deviation from expected titer |
Specimen and Sampling Consideration
| Aspect | FDA-Validated Requirement (Quantitative Syphilis Assays) |
| Specimen Type | Human serum or plasma; whole blood if validated. |
| Population | Adults, antenatal women, and individuals in follow-up or under treatment. |
| Sample Size | ≥500 samples; sufficient positive and negative representation. |
| Positive Samples | ≥75–100 covering full titer range and disease stages. |
| Negative Samples | 100–200 confirmed negatives by treponemal tests. |
| Cross-Reactive Samples | ≥50 with related infections or autoimmune markers. |
| Serial / Paired Samples | Paired pre- and post-treatment specimens verifying expected titer decline. |
| Storage / Stability | 2–8°C (≤72h) or −20°C (long-term). |
| Controls | Positive, negative, and mid-level controls per run. |
| Matrix Equivalence | ≥95% serum–plasma correlation. |
| Replicate Testing | Duplicate or triplicate runs for precision confirmation. |
Proper specimen quality is essential for reliable quantitative syphilis titer results. Degradation of reagin antibodies or improper handling may alter measured titers, leading to inaccurate assessment of disease activity or treatment response. Therefore, correct collection, storage, and transport conditions must be maintained to ensure consistent and reproducible quantitative performance.
| Test Objective | Minimum No. of Samples |
| Syphilis-Positive samples with established nontreponemal titers (confirmed by reference RPR/VDRL methods) | 50–100 |
| Syphilis-Negative samples | 100–200 |
| Potential Cross-reactive samples (e.g., HIV, autoimmune diseases, other STIs) | 20–30 |
| Total Clinical Specimens | 150–300 |
Syphilis-Positive Samples Should Represent
- A range of quantitative titers (low, moderate, high; including weakly reactive).
- Different infection stages (primary, secondary, early latent, late latent).
- Confirmed titer values by reference nontreponemal methods (RPR/VDRL).
- Pre- and post-treatment samples when assessing treatment-response claims.
Syphilis-Negative Samples Should Include
- Healthy individuals with no history of syphilis.
- Individuals with conditions associated with biological false positives (e.g., HIV, autoimmune disease, pregnancy, other STIs).
Additional Notes
- Sampling requirements may vary per intended use and IFU.
- Automated assays should include specimens challenging linearity, precision, hook effect, and carryover.
- Use of calibrated reference materials is recommended to ensure titer traceability across platforms.
Performance Criteria and Acceptance Standards
| Parameter | FDA Expectation / Typical Acceptance Standard |
| Limit of Quantitation (LoQ) | CV ≤ 20% and bias ≤ ±10% at the lowest measurable titer. |
| Precision / Reproducibility | CV ≤ 10% or ≥95% titer concordance across sites, days, and operators. |
| Accuracy / Method Comparison | Correlation vs. predicate quantitative titers ≥95%; bias within ±1 dilution or ±15%. |
| Linearity / Dynamic Range | R² ≥ 0.98 for proportional response across serial dilutions; slope 0.9–1.1. |
| Interference Testing | ≤5% deviation or ≤2% false reactivity when testing hemolysis, lipemia, bilirubin, etc. |
| Titer Concordance / Follow-up | Paired samples must confirm expected titer decline (e.g., fourfold reduction after treatment). |
| Stability Studies | Reagents: performance within ±10% of baseline. Specimens: titer results within ±1 dilution of initial values. |
Quantitative Syphilis Testing Algorithm
Software Automation and Cyber security
Automated or software-driven syphilis test systems must undergo thorough validation to ensure reliable operation, data accuracy, and secure handling of patient information. Software components should be developed and maintained in accordance with IEC 62304 for medical device software lifecycle processes, including risk management, verification, and change control. In addition, systems must address FDA cybersecurity guidance by implementing safeguards such as access controls, secure data transmission, audit trails, and protection against unauthorized intrusion. Together, these measures ensure software integrity, operational continuity, and the protection of sensitive health data throughout the device’s use.
| Parameter | Description | Requirement |
| Software Lifecycle | Validation and version control for automated readers. | Compliance with IEC 62304; documented traceability matrix. |
| Data Integrity | Secure electronic record management. | 21 CFR Part 11 compliant (audit trails, restricted access). |
| Risk Management | Assessment of software or automation-related hazards. | Risk control per ISO 14971. |
| Cybersecurity | Data encryption, authentication, and patch management. | FDA Premarket Cybersecurity Guidance (2023). |
Clinical Studies
Clinical performance evaluation is generally required for quantitative syphilis test kits intended for diagnostic use under FDA 510(k), especially when analytical validation alone does not fully demonstrate reliability of reported titers. Clinical studies must show how accurately the test measures antibody titers in real patient samples compared with an FDA-cleared quantitative reference method (e.g., quantitative RPR). Performance is typically evaluated using regression correlation, Bland–Altman bias analysis, and agreement at clinically relevant titer thresholds, with acceptance criteria such as strong correlation (R² ≥ 0.95) and minimal bias.
Clinical studies should include a representative mix of infection stages (early, late, previously treated, suspected reinfection) and potential cross-reactive conditions to ensure applicability in routine clinical settings. Existing FDA-cleared quantitative assays showing high correlation and low bias may support discussion with FDA to optimize clinical study size and design. Therefore, obtaining FDA Q-Submission feedback before starting clinical performance studies is recommended to confirm comparator methods, statistical targets, and cohort requirements.
Conclusion
Quantitative syphilis assays play a crucial role in assessing infection severity, monitoring treatment response, and detecting reinfection. As FDA Class II devices requiring 510(k) clearance, manufacturers must demonstrate strong analytical, scientific, and clinical performance. These tests provide accurate and reproducible titer measurements, supporting evidence-based management of Treponema pallidum infection.