Abstract
Designing an effective HIV-1 envelope glycoprotein (Env) immunogen for elicitation of broadly neutralizing antibodies (bNAbs) is a challenging task because of the high sequence diversity, heavy glycosylation, and inherent meta-stability of Env. Based on the antigenic profile of recently isolated bNAbs, the rational approach to immunogen design is to make a stable version of the Env trimer, which mimics the native trimeric Env present on the viral surface. The SOSIP.664 form of a clade A Env, BG505, yields a homogeneous and well ordered prefusion trimeric form, which maintains structural integrity and desired antigenicity. Following the same approach, we attempted to stabilize a naturally occurring efficiently cleaved clade C Env, namely 4-2.J41, isolated from an Indian patient. Although the SOSIP form of 4-2.J41 failed to produce reasonably well ordered trimers, the 4-2.J41.SOSIP.664 Env could be stabilized in a native-like trimeric form by swapping a domain from BG505 Env to 4-2.J41 Env. Using various biochemical and biophysical means we confirmed that this engineered Env is cleaved, trimeric, and it retains its native-like quaternary conformation exposing mostly broadly neutralizing epitopes. Moreover, introduction of a disulfide bond in the bridging sheet region further stabilized the closed conformation of the Env. Thus, our 4-2.J41.SOSIP.664 Env adds to the increasing pool of potential immunogens for a HIV-1 vaccine, particularly for clade C, which is the most prevalent in India and many other countries. Besides, the approach used to stabilize the 4-2.J41 Env may be used successfully with Envs from other HIV-1 strains as well. Additionally, a soluble native trimeric form of an efficiently cleaved membrane-bound Env, 4-2.J41, may be beneficial for immunization studies using various prime-boost strategies.
Highlights
Designing an effective HIV-1 envelope glycoprotein (Env) immunogen for elicitation of broadly neutralizing antibodies is a challenging task because of the high sequence diversity, heavy glycosylation, and inherent meta-stability of Env
The diffused electron density of the heptad repeat 1 (HR1) region of BG505 and JRFL Envs in two instances allows to trace the atomic coordinates and build-up the side chain rotamers with some degree of confidence [3, 25]
The SOSIP.664 trimeric form of clade A Env BG505, and clade B Env B41, show almost similar antigenic profiles corresponding to Env spikes on the viral surface [13, 36]
Summary
Envelope glycoprotein; bNAb, broadly neutralizing antibody; SEC, Size exclusion chromatography; NS-EM, negative stain electron microscopy; BLI, biolayer light interferometry; DSC, differential scanning calorimetry; gp, glycoprotein; IP, immunoprecipitation; VLP, virus-like particle. A disulfide linkage between residue 501 of gp120 and 605 of gp (SOS) stabilizes the trimeric conformation, whereas the isoleucine to proline substitution (I559P) in the heptad repeat 1 (HR1) region stabilizes the Env in its prefusion state [13] Envs expressed from this construct are known as SOSIP.664. We focused our effort on designing an immunogen with our previously identified membrane-bound efficiently cleaved clade C Env, 4-2.J41, of Indian origin. This envelope was of particular interest to us as it binds efficiently to bNAbs but poorly to non-NAbs when expressed on the cell surface [19, 20]. The stability of the trimer at physiological temperature and its high melting temperature makes it a suitable candidate immunogen for testing for prime-boost immunization studies and for structural analysis
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