Development of Fluorescently Labeled Self-Emulsifying Drug Delivery Systems (SEDDS) for Prolonged Stability, In Vitro Sustained Release, and Cellular Uptake

Ahmad Saleh Malkawi; Razan Haddad; Azhar Malkawi; Nasr Alrabadi

doi:10.2174/2211738510666220314103400

Development of Fluorescently Labeled Self-Emulsifying Drug Delivery Systems (SEDDS) for Prolonged Stability, In Vitro Sustained Release, and Cellular Uptake

Pharm Nanotechnol. 2022;10(2):146-161. doi: 10.2174/2211738510666220314103400.

Authors

Ahmad Saleh Malkawi^{1

2}, Razan Haddad³, Azhar Malkawi³, Nasr Alrabadi⁴

Affiliations

¹ Faculty of Pharmacy, Cyprus International University, Nicosia 99258 Cyprus.
² Department of Pharmaceutical Sciences, Faculty of Pharmacy, Isra University, Queen Alya Airport Street, Amman 11622 Jordan.
³ Department of Pharmaceutical Technology, Faculty of Pharmacy, Jordan University of Science and Technology, Irbid 22110 Jordan.
⁴ Department of Pharmacology, Faculty of Medicine, Jordan University of Science and Technology, Irbid 22110 Jordan.

PMID: 35289258
DOI: 10.2174/2211738510666220314103400

Abstract

Aims: In this study, four fluorescein hydrophobic ionic complexes were formed with the cationic polymers Eudragit RS, Eudragit RL, Eudragit E, and polyethyleneimine (PEI) to provide fluorescein sustained release, sustained cellular uptake, and stability.

Methods: Complexes were loaded in a self-emulsifying drug delivery system (SEDDS) composed of 40% Tween 80, 20% Kolliphor EL, 15% 2-n-Octyl-1-dodecanol, and 25% dipropylene glycol. SEDDS were investigated regarding their size, polydispersity index (PDI), zeta potential, and cytotoxicity. Fluorescein release from SEDDS was performed in phosphate buffer (pH 6.8 and pH 8), and the released fluorescein was evaluated for cellular uptake. Moreover, fluorescein from all of the SEDDS pre-concentrates was released at different time points to check its long-term stability over six months.

Results: The average fluorescein load in SEDDS was 0.045%. SEDDS showed an average droplet size of 24.9 ± 1.6 nm with PDI ≤ 0.3. SEDDS complexes diluted 1:100 increased the zeta potential from -7.3 mV to +3.7 mV and provided > 85% cell viability. A 92.27 ± 3.18% fluorescein exhibited a few seconds of immediate release when used as control or PEI complex in SEDDS. On the contrary, Eudragit-fluorescein complexes in SEDDS showed sustained release of 87.01 ± 5.22% fluorescein in ≤ 70 min with 22.19 ± 14.56% and 59.27 ± 16.57% released at 10 min in pH 6.8 and pH 8 release media, respectively. Comparatively, the medium at pH 6.8 maintained a significantly improved sustained fluorescein release (p ≤ 0.001). Furthermore, Eudragit RS/RL compared to Eudragit E, significantly exhibited a slower fluorescein release rate from SEDDS (p ≤ 0.01). The cellular uptake of the released fluorescein was 72.4 ± 8.2% for all SEDDS complexes after 3 h. Eudragit complexes compared to PEI complex in SEDDS significantly showed m ore sustained fluorescein cellular uptake at 1 h and 2 h (p ≤ 0.001). However, SEDDS complexes showed the longest fluorescein stability with PEI after six months, whereas fluorescein stability for SEDDS containing fluorescein as Eudragit complex and control showed 39.1% and 82.5% fluorescence decrease, respectively, after three months.

Conclusion: In the developed SEDDS, the presence of hydrophobic ionic complexes can significantly promote longer stability and sustained cellular uptake of fluorescein while releasing in a sustained manner.

Keywords: Hydrophobic ion pairing; SEDDS; dielectric constant; fluorescein; nanoemulsions; sustained release.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Delayed-Action Preparations
Drug Delivery Systems*
Emulsions / chemistry
Fluoresceins
Hydrophobic and Hydrophilic Interactions

Substances

Delayed-Action Preparations
Emulsions
Fluoresceins