# Biochemistry of Intrinsic Xase

> **NIH NIH P01** · CHILDREN'S HOSP OF PHILADELPHIA · 2022 · $732,776

## Abstract

Project 4 - Abstract
Novel approaches to enhance the biologic activity of FVIII and FIX are critical endeavors with potential for
improving protein- and gene-based therapy for hemophilia. We have identified novel variants and new
strategies that have a positive effect on the biological activity of FVIII and FIX. Promising preclinical studies on
efficacy and safety in small and large animal models provide the basis for translational studies using these
proteins; in particular the FIX-Padua (R338L) variant is already in early phase gene therapy clinical trials for
hemophilia B. The main goal of this application is to understand the biochemistry of the variants and in the
case of new variants, evaluate their potential in hemophilic models. We seek to use this approach to reveal
mechanistic aspects of intrinsic Xase function and thus provide evidence-based insights into the potential of
these variants in the treatment of human disease. The central tenets of our experimental strategies are based
on the fact that even modest enhancements of procoagulant function, as judged from a biochemical
perspective, can have a very significant impact on the success of therapeutic approaches. In aim 1 we
hypothesize that a FVIII derivative with a modified PACE/furin cleavage site results in its differential processing
by thrombin and/or FXa yielding a more stable/active cofactor. A second class of variant is based on a
molecule lacking the B-domain and acid region 3 with increased specific activity. These findings pose the
question whether vWF engagement, while an important determinant of FVIII circulating half-life, limits
activation by FXa, and if by relieving this constraint we can enhance available FVIIIa levels to promote clot
formation. In aim 2 we will characterize the FIX-Padua variant for which the molecular basis for its enhanced
function is uncertain. We will use biochemical and biophysical approaches to identify the mechanism of the
hyperfunctional molecule. Emerging structural information derived from FXa aptamers that prevent its binding
to FVa and the known structure of snake FVa-FX implicate a region of Xa not previously considered central in
Va binding. We hypothesize that the analogous interaction between FIXa and FVIIIa may be enhanced by
modifications in the heparin-binding exosite. If successful, our goal is to combine FIX-Padua with modifications
from the FIX-loop 90 to generate FIX variants with enhanced biologic properties. In aim 3 we will pursue
studies with variants of FIX that upon activation yield products with increasing zymogen-like character, are
long-lived because of their resistance to protease inhibition but may be functionally rescued upon their
assembly into the intrinsic Xase. Biochemical studies testing these ideas will be followed by approaches to
assess if such variants, and those combined on the FIX-Padua background, have therapeutic value for
hemophilia B. Together these approaches will provide new mechanistic insights int...

## Key facts

- **NIH application ID:** 10439608
- **Project number:** 5P01HL139420-05
- **Recipient organization:** CHILDREN'S HOSP OF PHILADELPHIA
- **Principal Investigator:** Valder R. Arruda
- **Activity code:** P01 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2022
- **Award amount:** $732,776
- **Award type:** 5
- **Project period:** 2018-09-01 → 2024-06-30

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/10439608

## Citation

> US National Institutes of Health, RePORTER application 10439608, Biochemistry of Intrinsic Xase (5P01HL139420-05). Retrieved via AI Analytics 2026-05-24 from https://api.ai-analytics.org/grant/nih/10439608. Licensed CC0.

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