Study on stabilized mechanism of high internal phase Pickering emulsions based on commercial yeast proteins: Modulating the characteristics of Pickering particle via sonication

Tianfu Cheng; Guofang Zhang; Fuwei Sun; Yanan Guo; Ramnarain Ramakrishna; Linyi Zhou; Zengwang Guo; Zhongjiang Wang

doi:10.1016/j.ultsonch.2024.106843

Study on stabilized mechanism of high internal phase Pickering emulsions based on commercial yeast proteins: Modulating the characteristics of Pickering particle via sonication

Ultrason Sonochem. 2024 Mar:104:106843. doi: 10.1016/j.ultsonch.2024.106843. Epub 2024 Mar 8.

Authors

Tianfu Cheng¹, Guofang Zhang¹, Fuwei Sun¹, Yanan Guo¹, Ramnarain Ramakrishna², Linyi Zhou³, Zengwang Guo⁴, Zhongjiang Wang⁵

Affiliations

¹ College of Food Science, Northeast Agricultural University, Harbin, Heilongjiang 150030, China.
² Department of Plant Sciences, North Dakota State University, Fargo, ND 58108, USA.
³ College of Food and Health, Beijing Technology and Business University, Beijing 100048, China.
⁴ College of Food Science, Northeast Agricultural University, Harbin, Heilongjiang 150030, China. Electronic address: gzwname@163.com.
⁵ College of Food Science, Northeast Agricultural University, Harbin, Heilongjiang 150030, China; National Grain Industry Technology Innovation Center, Harbin, Heilongjiang 150030, China. Electronic address: wzjname@126.com.

Abstract

The primary significance of this work is that the commercial yeast proteins particles were successfully used to characterize the high internal phase Pickering emulsions (HIPPEs). The different sonication time (0,3,7,11,15 min) was used to modulate the structure and interface characteristics of yeast proteins (YPs) that as Pickering particles. Immediately afterward, the influence of YPs particles prepared at different sonication time on the rheological behavior and coalescence mechanism of HIPPEs was investigated. The results indicate that the YPs sonicated for 7 min exhibited a more relaxed molecular structures and conformation, the smallest particle size, the highest H₀ and optimal amphiphilicity (the three-phase contact (θ) was 88.91°). The transition from extended to compact conformations of YPs occurred when the sonication time exceeded 7 min, resulting in an augmentation of size of YPs particles, a reduction in surface hydrophobicity (H₀), and an elevation in hydrophilicity. The HIPPEs stabilized by YPs particles sonicated for 7 min exhibited the highest adsorption interface protein percentage and a more homogeneous three-dimensional (3D) protein network, resulting in the smallest droplet size and the highest storage (G'). The HIPPEs sample that stabilized by YPs particles sonicated for 15 min showed the lowest adsorption protein percentage. This caused a reduction in the thickness of its interface protein layer and an enlargement in the droplet diameter (D _[3,2]). It was prone to droplet coalescence according to the equation used to evaluate the coalescence probability of droplets (Eq (2)). And the non-adsorbed YPs particles form larger aggregation structures in the continuous phase and act as "structural agents" in 3D protein network. Therefore, mechanistically, the interface protein layer formed by YPs particles sonicated 7 min contributed more to HIPPEs stability. Whereas the "structural agents" contributed more to HIPPEs stability when the sonication time exceeded 7 min. The present results shed important new light on the application of commercial YPs in the functional food fields, acting as an available and effective alternative protein.

Keywords: Coalescence; High internal phase Pickering emulsions; Particle; Sonication; Yeast proteins.

MeSH terms

Emulsions / chemistry
Fungal Proteins*
Hydrophobic and Hydrophilic Interactions
Particle Size
Sonication*

Substances

Emulsions
Fungal Proteins