Beer consumption and changes in stability of human serum proteins

Shela Gorinstein*, Abraham Caspi, Ivan Goshev, Snejana Moncheva, Marina Zemser, Moshe Weisz, Imanuel Libman, Henry Tzvi Lerner, Simon Trakhtenberg, Olga Martín-Belloso

*Corresponding author for this work

Research output: Contribution to journalArticlepeer-review

9 Scopus citations

Abstract

The aim of this study was to evaluate the influence of beer consumption (BC) on the functional and structural properties of human serum proteins (HSP). Thirty-eight volunteers (after coronary bypass) were divided into two groups: experimental (EG) and control (CG). Nineteen volunteers of the EG consumed 330 mL per day of beer (about 20 g of alcohol) for 30 consecutive days. The CG volunteers consumed mineral water instead of beer. Blood samples were collected from EG and CG patients before and after the experiment. Albumin (Alb), globulin (Glo), and methanol-precipitable proteins (MPP) from human serum were denatured with 8 M urea. Fluorescence and electrophoresis were employed in order to elucidate urea-induced conformational changes and structural behavior of proteins. The measured fluorescence emission spectra were used to estimate the stability of native and denatured protein fractions before and after BC. It was found that before BC the fractions most stable to urea denaturation were Glo, Alb, and MPP fractions. After BC in most of the beer-consuming patients (EG) some changes in native and denatured protein fractions were detected: a tendency to lower stability and minor structural deviations. These qualitative changes were more profound in MPP than in Alb and Glo. Thus, Glo is more resistible to alcohol influence than Alb, which in turn is more resistible than MPP. No serum protein changes were detected in patients of CG.

Original languageEnglish
Pages (from-to)1441-1445
Number of pages5
JournalJournal of Agricultural and Food Chemistry
Volume49
Issue number3
DOIs
StatePublished - 2001

Keywords

  • Beer consumption
  • Denaturation
  • Electrophoresis
  • Fluorescence
  • Human serum proteins

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