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Spectroscopic Investigation of Losartan and Glipizide Competitive Binding to Glycated Albumin in Polypharmacotherapy: A Comparative Study

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Abstract
Understanding the interaction between pharmaceuticals and serum proteins is crucial for optimizing therapeutic strategies, especially in patients with coexisting chronic diseases. The primary goal of this study was to assess the potential changes in binding affinity and competition between glipizide (GLP, a second-generation sulfonylurea hypoglycemic drug) and losartan (LOS, a medication commonly prescribed for hypertension, particularly for patients with concurrent diabetes) with non-glycated (HSA) and glycated (gHSAGLC, gHSAFRC) human serum albumin using multiple spectroscopic techniques (fluorescence, UV-visible absorption, and circular dichroism spectroscopy). The results indicate that FRC is a more effective glycation agent for HSA than GLC, significantly altering the albumin structure and affecting the microenvironment around critical amino acid residues, Trp-214 and Tyr. These modifications reduce the binding affinity of LOS and GLP to gHSAGLC and gHSAFRC, compared to HSA, resulting in less stable drug-protein complexes. The study reveals that LOS and GLP interact nonspecifically with the hydrophobic regions of the albumin surface in both binary (ligand-albumin) and ternary systems (ligand-albumin-ligandconst) and specifically saturate the binding sites within the protein molecule. Furthermore, the presence of an additional drug (GLP in the LOS-albumin complex or LOS in the GLP-albumin complex) complicates the interactions, likely leading to competitive binding or displacement of the initially bound drug in both non-glycated and glycated albumins. Analysis of the CD spectra suggests mutual interactions between GLP and LOS, underscoring the importance of closely monitoring patients co-administered these drugs to ensure optimal therapeutic efficacy and safety. Początek formularzaDół formularza
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Subject: Medicine and Pharmacology  -   Pharmacy

1. Introduction

The escalating prevalence of chronic diseases, including hypertension and type 2 diabetes mellitus, has necessitated the widespread use of polypharmacotherapy. This therapeutic approach mandates a comprehensive understanding of drug interactions and their biochemical implications, mainly when pharmaceuticals interact with modified biological molecules such as glycated human serum albumin (gHSA). gHSA, a product of non-enzymatic glycation of human serum albumin (HSA), is prevalent in diabetic patients and has significant clinical implications due to its altered structure, biological function, and physicochemical properties [1,2].
Albumin, the primary protein in human plasma, is essential for maintaining oncotic pressure and transporting various endogenous and exogenous substances. Furthermore, HSA possesses anti-inflammatory, antioxidant, and antithrombotic properties [3]. Under diabetic conditions, HSA undergoes glycation, which can markedly affect its drug-binding capabilities. Glycated albumin serves not only as a marker of short-term glycemic control but also influences the pharmacokinetics and pharmacodynamics of therapeutic agents, potentially altering their efficacy and safety profiles [4]. Understanding how glycation modifies albumin's binding properties is essential for optimizing drug dosing and minimizing adverse effects in diabetic patients.
Losartan (LOS, Figure 1a) is widely used for its antihypertensive properties, primarily by inhibiting the renin-angiotensin system. By blocking angiotensin II from binding to the AT1 receptor, LOS induces vasodilation and decreases aldosterone secretion, lowering blood pressure [5,6]. LOS exhibits a high affinity to HSA, predominantly binding at site II, also known as the benzodiazepine-binding site [7]. This significant binding within subdomain IIIA of the HSA macromolecule ensures that a considerable portion of LOS remains inactive in the bloodstream, with only a minor fraction available as a free drug to exert its therapeutic effects.
Glipizide (GLP, Figure 1b), a second-generation sulfonylurea, is widely used to manage blood glucose levels in patients with type 2 diabetes mellitus. It exerts its pharmacological effects by stimulating insulin secretion from pancreatic β-cells. This is achieved by inhibiting ATP-sensitive potassium channels on the β-cell membrane, leading to membrane depolarization and subsequent insulin release, thereby reducing blood glucose levels [8]. The study using high-performance affinity chromatography (HPAC) revealed that GLP interacts with both Sudlow's sites I and II on HSA but with greater affinity for site II than the site I [9]. Anwer et al. performed molecular docking and simulation studies in silico, showing that the glipizide-HSA complex is formed due to hydrogen bonds and hydrophobic interactions [8].
In combination therapy, LOS and GLP may compete for the same binding site on HSA. This competitive binding can influence their pharmacokinetics and pharmacodynamics, potentially affecting their efficacy and safety profiles. The primary aim of this study was to compare the interactions of losartan and glipizide with human serum albumin– both non-glycated (HSA) and glycated by glucose (gHSAGLC) and fructose (gHSAFRC)– and to investigate their mutual binding interactions using spectroscopic techniques (fluorescence spectroscopy, UV-visible absorption spectroscopy, and circular dichroism spectroscopy – CD). These techniques are widely recognized for studying in vitro interactions of drugs with albumin due to their sensitivity, speed, and simplicity [10,11,12]. They are beneficial for calculating binding and quenching parameters, mean residue ellipticity, and characterizing proteins’ secondary and tertiary structures.
By elucidating the competitive binding interactions of LOS and GLP with glycated albumin at a molecular level, this research seeks to provide insights that could inform better clinical practices in polypharmacotherapy, particularly for patients at risk of altered drug efficacy due to glycation. This understanding is imperative for optimizing therapeutic strategies in patients with comorbid hypertension and diabetes.

2. Results and Discussion

2.1. HSA Glycation – Formation of Glycation Products

Reducing sugars, such as glucose (GLC) and fructose (FRC), react with the primary free amino groups of the NH2-terminal amino acid and/or the ε-amino group of lysine (Lys), arginine (Arg), and the thiol group of cysteine (Cys-34), leading to their glycation. The final stage of this process is the formation of AGEs – Advanced Glycation End-products, a heterogeneous group of compounds considered a critical pathophysiological factor in diabetic complications [13]. In vitro studies utilize various glycation agents and specific experimental conditions to initiate the glycation process. GLC, the most abundant sugar in the human body, plays a critical role in the endogenous formation of AGEs and serves as an essential biomarker in the assessment of diabetes. However, recent research has demonstrated that diabetes is also associated with abnormal fructose metabolism. Uric acid, produced from endogenous fructose, can lead to kidney and cardiovascular disease, hypertension, and obesity in diabetic patients, as FRC is generated via the polyol pathway [14,15]. Accordingly, glucose, the body's primary energy source, and fructose, a dietary reducing sugar, were prompted to be used as glycation agents for human serum albumin (HSA) under in vitro conditions.
A comparative analysis of the emission fluorescence spectra of glycation products formed in glycated albumin (gHSAGLC, gHSAFRC) and those present in non-modified HSA showed a significant increase in the fluorescence intensity of AGEs in the glycated proteins upon excitation at λex = 335 nm (Figure 2a) and λex = 485 nm (Figure 2b).
From the experiment results, it is evident that FRC induces glycation of HSA more effectively than GLC. The higher fluorescence intensity of AGEs observed in gHSAFRC suggests that HSA undergoes a faster and more efficient Amadori rearrangement in the presence of FRC than in the HSA-GLC system. In addition to the hyperchromic effect, this study observed a hypsochromic shift of the fluorescence maxima of glycated albumin AGEs compared to HSA excited at λex = 335 nm (Δλmax = 6 nm). This blue shift indicates a decrease in polarity within the environment of the newly formed products (Figure 2a). Irradiation in the wavelength ranges of 320 nm to 335 nm and 325 nm to 335 nm causes the excitation of argpyrimidine (AP) and pentosidine (PEN), respectively. These compounds, which exhibit fluorescent properties, are formed due to protein modifications by methylglyoxal through interactions with arginine residues in macromolecules [16]. AP emits fluorescence at an approximate wavelength of λem ~ 400 nm, while PEN in the range of λem = 375 nm to 385 nm [17]. The glycated albumin products gHSAGLC and gHSAFRC, when excited at λex = 335 nm (Figure 2a), do not display fluorescence typical of PEN and AP. The fluorescence of AGEs at around λem = 420 nm suggests the formation of PEN and AP in glycated proteins but also indicates the presence of additional fluorophores. This is evidenced by the shift of the fluorescence maximum towards longer wavelengths compared to the emission of PEN and AP, as described by Kessel et al. [17]. An advantage of measurements at λex = 485 nm is the absence of interference from other fluorophores in the sample. According to Schmitt et al., fluorescence with an emission maximum at λem = 530 nm (Figure 2b) appears to be an indicator of arginyl residue modifications [18]. The results presented here confirm the efficacy of the glycation process under the experimental conditions applied in this study, providing a solid foundation for further research in this area.

2.2. Investigating the Interaction of Losartan and Glipizide with Non-Glycated and Glycated Human Serum Albumin in Binary and Ternary Complexes

Assessing changes in the fluorescence emission intensities of aromatic amino acid residues within proteins can effectively reveal intermolecular interactions [19]. Human serum albumin (HSA) contains 18 fluorescent tyrosine residues (Tyr-9, Tyr-39, Tyr-84, Tyr-138, Tyr-140, Tyr-148, Tyr-150, Tyr-161, Tyr-263, Tyr-319, Tyr-332, Tyr-334, Tyr-340, Tyr-341, Tyr-372, Tyr-375, Tyr-401, Tyr-411), along with a single, strongly fluorescent tryptophan residue (Trp-214) buried within a hydrophobic pocket [20]. The fluorescence quenching technique is commonly employed to determine the strength and mechanism of interactions between ligands (drugs) and albumin, especially involving the Trp-214 and Tyr residues located within albumin's subdomains IIA and/or IB, IIB, and IIIA.
Fluorescence quenching of non-glycated (HSA) and glycated (gHSAGLC, gHSAFRC) albumin, excited at λex = 275 nm and λex = 295 nm, was performed to determine the interaction of losartan (LOS) and glipizide (GLP) at high-affinity binding sites of albumins in the binary systems: LOS-HSA (Figure 3a), LOS-gHSAGLC (Figure 3b), LOS-gHSAFRC (Figure 3c), GLP-HSA (Figure 3d), GLP-gHSAGLC (Figure 3e), GLP-gHSAFRC (Figure 3f).
In fluorescence studies, attention is directed towards specific protein regions containing fluorophores. Using an excitation wavelength of 275 nm enables the observation of both tryptophan (Trp-214) and tyrosine (Tyr) residues, whereas a 295 nm wavelength selectively excites Trp-214 due to its unique spectral characteristics. The primary drug-binding sites are located within the IIA and IIIA subdomains of HSA. Both hydrophobic pockets contain at least one type of the mentioned amino acids, which can transfer energy to a ligand if it is close to the fluorophore [21].
In Sudlow's site I, located in the IIA subdomain, one tryptophan (Trp-214) and one tyrosine (Tyr-263) residue can participate in drug binding. Although Trp-214 is the sole tryptophan in the HSA structure, it plays a vital role in ligand interactions. The IIIA subdomain includes three tyrosine residues (Tyr-401, Tyr-411, and Tyr-497), which can transfer energy to the acceptor [22]. Additionally, Tyr-401 and Tyr-411 have been identified as amino acids that stabilize the binding of numerous ligands. To verify subdomain IIIA of human serum albumin as the specific binding site for LOS and GLP, quenching curves of HSA, gHSAGLC and gHSAFRC excited at λex = 275 nm were compared with those excited at λex = 295 nm with the addition of LOS (Figure 3a–c) and GLP (Figure 3d–f) at increasing concentrations.
As mentioned earlier, protein fluorescence quenching occurs when the distance between the chromophores in the aromatic rings of the ligand's chemical structure and the fluorophores of albumin is less than 10 nm according to Stryer [23] and less than 7 nm according to Valeur [21]. This proximity enables fluorescence resonance energy transfer (FRET) from a donor (fluorophore) to an acceptor (chromophore), leading to non-radiative, direct energy transfer to the drug molecule. The quenching curves of HSA (Figure 3a,d), gHSAGLC (Figure 3b,e) and gHSAFRC (Figure 3c,f) in the presence of both losartan and glipizide at increasing concentrations (with molar ratios of ligand to albumin from 1:1 to 10:1 for LOS and 1:1 to 5:1 for GLP) indicate a decrease in fluorescence for non-glycated and glycated albumin at excitation wavelengths of 275 nm and 295 nm. This indicates effective energy transfer between albumin fluorophores and the ligands. After applying corrections for the inner filter effect, the observed fluorescence quenching of HSA, gHSAGLC, gHSAFRC can be attributed to the formation of LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC and GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC complexes.
Based on the data collected in Table S1 (Supplementary Materials), the percentage of non-glycated HSA fluorescence quenching, used as a control albumin, is nearly similar, reaching approximately 49.20% and 45.17% for LOS and 57.86% and 51.46% for GLP at λex = 275 nm and λex = 295 nm, respectively. For glycated albumin, weaker fluorescence quenching was observed in the presence of increasing ligand concentrations compared to the control sample, with the weakest quenching seen for albumin glycated by fructose (gHSAFRC). LOS quenches the fluorescence of gHSAGLC by 41.67% at λex = 275 nm and by 33.36% at λex = 295 nm. The fluorescence of gHSAFRC decreases by 29.62% at 275 nm and by 16.54% at 295 nm for the same molar ratio of ligand to albumin (10:1). GLP quenches the fluorescence of gHSAGLC by 49.42% at λex = 275 nm and by 37.41% at λex = 295 nm, at molar ratio GLP:albumin 5:1. In contrast, the fluorescence of gHSAFRC at λex = 275 nm and λex = 295 nm decreases by 38.93% and 21.46%, respectively. Moreover, the data presented in Table S1 indicate that both LOS and GLP have a higher affinity towards non-glycated macromolecule than towards glycated proteins (gHSAGLC and gHSAFRC).
The quenching curves of albumins excited at λex = 275 nm and λex = 295 nm in the presence of LOS (Figure 3a–c) and GLP (Figure 3d–f) at increasing drug concentration do not overlap above the molar ratio LOS:HSA 2:1, LOS:gHSAGLC 1:1, LOS:gHSAFRC 1:1 and GLP:HSA 1.5:1, GLP:gHSAGLC 0.5:1. The exact course of fluorescence quenchning curves indicates that there is no difference in energy transfer between the tyrosyl residues and the ligand, suggesting that initially only Trp-214 residue is likely involved in the interaction with LOS and GLP. This may allow the identification of subdomain IIA as a high-affinity binding site in the albumin structure. In contrast, a different trajectory of fluorescence quenching suggests that both tryptophanyl residue in subdomain IIA and tyrosyl residues located in hydrophobic subdomains IB, IIB, IIIA, and IIIB are involved in the interaction with LOS and GLP in the binding site environment. As shown in Figure 3, the fluorescence quenching of HSA (Figure 3a,d), gHSAGLC (Figure 3b,e), and gHSAFRC (Figure 3c,f) by LOS and GLP is more pronounced when excited at λex = 275 nm compared to λex = 295 nm. This likely indicates a significant involvement not only of Trp-214 but also of Tyr residues in the interaction between the ligands and albumins.
The quenching curves of non-glycated and glycated albumin in the presence of LOS (Figure S1ab, Supplementary Materials) and GLP (Figure S1cd, Supplementary Materials) exhibit significant differences in their profiles. Specifically, these differences result from 7.53% and 11.81%, 19.58% and 28.63% lower quenching of gHSAGLC and gHSAFRC by LOS relative to the LOS-HSA system at λex = 275 nm and λex = 295 nm, respectively. For the GLP-gHSAGLC and GLP-gHSAFRC systems, the differences in the quenching curves profiles amount to 8.44% and 14.05% for gHSAGLC, and 18.93% and 30% for gHSAFRC relative to the GLP-HSA system at λex = 275 nm and λex = 295 nm, respectively (Table S1). Several factors may explain these observed differences. Glycation induces conformational changes in the albumin structure, modifying the binding sites and overall protein flexibility and affecting the interaction with quenchers. Additionally, glycation alters the microenvironment around crucial amino acid residues, such as Trp-214 and Tyr, influencing their accessibility to quenchers. The binding affinity of glycated albumin for LOS and GLP may also differ due to sugar moieties, which can either hinder or facilitate quencher binding [24]. Furthermore, steric hindrance from added sugar groups can reduce quenching efficiency, while new chemical interactions and potential protein aggregation further impact the quenching dynamics. These combined factors contribute to the distinct quenching behaviours observed for non-glycated and glycated albumin at different excitation wavelengths.
The influence of GLP on the LOS and LOS on the GLP affinity towards HSA, gHSAGLC and gHSAFRC was studied by comparing the quenching curves of albumins in the presence of LOS in the binary LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC and ternary complexes LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst (Figure 4), and in the presence of GLP in the binary GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC and ternary complexes GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst (Figure 5).
The fluorescence quenching observed in the LOS-HSA-GLPconst (Figure 4a,b), LOS-gHSAGLC-GLPconst (Figure 4c,d) and GLP-HSA-LOSconst (Figure 5a,b) systems differs from the quenching observed in the binary systems LOS-HSA (Figure 4a,b), LOS-gHSAGLC (Figure 4c,d) and GLP-HSA (Figure 5a,b), respectively. The quenching of HSA and gHSAGLC by LOS and HSA by GLP at maximum concentration is more pronounced by 11.64% (Figure 4a), 6.64% (Figure 4c), 16.69% (Figure 4b), 10.04% (Figure 4d), 11.76% (Figure 5a), and 17.7%% (Figure 5b) compared to the systems with an additional ligand added to the binary system. An additional pharmaceutical in the system likely complicates the interaction between LOS-HSA and LOS-gHSAGLC (or GLP-HSA) or interferes with forming these complexes. GLP (or LOS) may cause the displacement of LOS (or GLP) from its complex with non- and glycated HSA. This effect may arise from competitive binding sites on albumin, steric hindrance, or conformational alterations of the macromolecule induced by the binding of the second ligand. Furthermore, the differing affinities and binding dynamics of GLP and LOS for albumin could result in preferential binding of one ligand over the other, thereby influencing the observed quenching effect. In contrast, the absence of differences in the quenching of intrinsic fluorescence of glycated albumin by LOS or GLP in the binary systems LOS-gHSAFRC (Figure 4e,f), GLP-gHSAGLC (Figure 5c,d), and GLP-gHSAFRC (Figure 5e,f) compared to the ternary systems LOS-gHSAFRC-GLPconst (Figure 4e,f), GLP-gHSAGLC-LOSconst (Figure 5c,d), and GLP-gHSAFRC-LOSconst (Figure 5e,f) suggests that glycation, particularly glycation of albumin by fructose, alters the macromolecule's structure and/or binding characteristics. This modification prevents the additional drug – GLP in the LOS-gHSAFRC complex or LOS in the GLP-gHSAGLC and GLP-gHSAFRC complexes – from competing for the binding site with LOS and GLP and prevents the displacement of drugs already bound in the gHSAGLC and gHSAFRC molecules.
Additionally, the study on the LOS-HSA, LOS-gHSAGLC, GLP-HSA, and LOS-HSA-GLPconst system revealed that an increase in drug concentration leads to a hypsochromic shift (∆λmax) of the fluorescence emission band relative to the maximum emission of unbound albumin. The hypsochromic shift indicates an increase in the hydrophobic nature of the fluorophore environment due to drug interaction with albumin. It also suggests the possibility of hydrophobic interactions between the aromatic rings of LOS and GLP molecules and the aromatic rings of amino acid residues. The more pronounced hypsochromic shift upon excitation of albumin fluorescence at λex = 275 nm than at λex = 295 nm indicates a less polar environment not only around Trp-214 but also around tyrosyl residues. The more substantial ∆λmax shift towards the blue in the double systems compared to the triple systems, i.e., in the LOS-HSA system compared to LOS-HSA-GLPconst by 5 nm, LOS-gHSAGLC compared to LOS-gHSAGLC-GLPconst by 4 nm, and GLP-HSA compared to GLP-HSA-GLPconst by 6 nm, and for non-modified compared to glycated albumin, may indicate a decrease in the hydrophobic nature of the environment of tryptophan or/and tyrosyl residues of albumin after glycation and in the presence of an additional drug in the drug-albumin system.
The quenching mechanism of losartan and glipizide interaction with both non-glycated and glycated serum albumin was determined using the Stern-Volmer plots. The analysis encompassed the binary systems LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC (Figure 6a), GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC (Figure 6b), as well as the ternary systems LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst (Figure 6c), GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst (Figure 6d) at λex = 275 nm (Figure 6) and λex = 295 nm (Figure S2, Supplementary Materials).
The dependence of F 0 F on LOS or GLP concentration in the binary and ternary systems at λex = 275 nm (Figure 6) and λex = 295 nm (Figure S2, Supplementary Materials) demonstrated a linear correlation for ligand-albumin complexes. The linear Stern-Volmer plots for the ligand-albumin and ligand-albumin-ligandconst system may indicate a dynamic (collisional) or static quenching mechanism of fluorescence for both non-modified (HSA) and glycated albumins (gHSAGLC, gHSAFRC). According to the literature, the ligand penetrates the macromolecule's environment in dynamic quenching, and fluorescence quenching is caused by the collision between the quencher molecule and the albumin fluorophore(s). In contrast, static quenching leads to a decrease in the intensity of emitted fluorescence when the ligand binds to the fluorophore molecule in its ground (non-excited) state, thereby reducing the population of fluorophores capable of being excited [25].
Table 1 and Table 2 present the Stern-Volmer constants K S V , the bimolecular quenching rate constant k q , and the fractional accessible protein fluorescence f a calculated for binary (ligand-albumin) and ternary (ligand-albumin-ligandconst) systems at λex = 275 nm and λex = 295 nm.
The magnitude of the determined fluorescence quenching rate constants k q ​ (10¹²) for the investigated systems indicates a static fluorescence quenching mechanism in the LOS-albumin, LOS-albumin-GLPconst (Table 1) and GLP-albumin, GLP-albumin-LOSconst systems (Table 2). According to Lakowicz, for collisional fluorescence quenching, the maximum value of the constant k q ​ in an aqueous solution is 2 × 10¹⁰ (L∙mol−1∙s−1) [27].
The Stern-Volmer constant serves as a means to assess the accessibility of the quencher to the excited fluorophore. A higher K S V   value indicates a greater availability of ligand molecules in the macromolecule, which leads to the formation of a complex in the excited state [28]. Glycation of HSA by glucose and fructose results in a decrease in the Stern-Volmer constant in both binary (LOS-albumin, GLP-albumin) and ternary systems (LOS-albumin-GLPconst) at excitation wavelengths of 275 nm and 295 nm. This indicates a lower quenching efficiency of glycated albumin fluorophores compared to non-modified albumin by losartan (Table 1). In the ternary system (GLP-albumin-LOSconst), fructose-induced glycation decreased K S V , whereas glucose-induced glycation increased K S V (Table 2). The K S V values determined for the system in the presence of an additional drug (LOS-albumin-GLPconst) are higher than those for the LOS-albumin system, both for unmodified and glycated albumin at λex = 275 nm. At λex = 295 nm, the same effect of increasing K S V is observed only for the system with glycated albumin, while the presence of GLP in the LOS-HSA system caused a slight decrease in K S V (Table 1). Conversely, the K S V values determined for the system in the presence of an additional drug (GLP-albumin-LOSconst complex) are lower for HSA and gHSAGLC at λex = 275 nm and λex = 295 nm. In contrast, for gHSAFRC, they remain unchanged at λex = 275 nm or are higher at λex = 295 nm (Table 2). At both excitation wavelengths (λex = 275 nm and λex = 295 nm), GLP complexes exhibit higher K S V values than to LOS complexes, indicating greater quenching efficiency. GLP molecules are closer to fluorophores of non-modified and glycated albumin than LOS molecules in binary and ternary complexes. It is also observed that K S V values are generally higher at λex = 275 nm compared to λex = 295 nm. The bimolecular quenching rate constants ( k q ) align with the trends observed in K S V . Most complexes display fractional accessibility ( f a ) close to or equal to 1, suggesting near-complete accessibility of the fluorophore to the quencher, with GLP-HSA showing the lowest accessibility (Table 2 ).
The nature of ligand binding to albumin (specificity of binding sites within the various classes of binding sites) was determined based on the binding isotherms (saturation curves) of LOS and GLP to non-glycated and glycated HSA in binary (Figure 7 ab) and ternary systems (Figure 7cd).
For LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC (Figure 7a), GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC (Figure 7b), LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst (Figure 7c) and GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst (Figure 7d) complexes at λex = 275 nm (Figure 7) and at λex = 295 nm (Figure S3, Supplementary Materials), the course of the saturation curves is not linear across the entire range of ligand concentrations, as each of the binding isotherms exhibits an exponentially increasing course and does not reach a "plateau". Therefore, based on the analyzed plots, it can be inferred that LOS and GLP nonspecifically interact with the hydrophobic fragments of the surface of non-glycated and glycated albumin in both binary and ternary systems and specifically saturate the binding sites within the protein molecule, as confirmed by the literature [29]. Specific binding is characterized by high affinity and low binding capacity, whereas nonspecific binding is characterized by low affinity and unlimited ligand binding capacity of the ligand [29]. The physicochemical compatibility of both molecules determines the binding of ligands to serum albumin. Small structural changes in the protein molecule can influence the mutual interaction of the drug with albumin, which in turn affects the binding parameters.
Specific binding of losartan and glipizide to non-modified and glycated albumin in the complexes LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC, GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC, LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst and GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst were quantitatively analyzed by calculating the association constant K a using the Scatchard equation (with ligand-bound fraction concentration as the independent variable) (Figure 8), the Klotz equation (with the inverse of the free ligand fraction concentration as the independent variable) (Figure 9), and through non-linear regression based on the Levenberg-Marquardt algorithm, i.e., binding isotherms (Figure 7). Additionally, Hill's coefficients ( n H ) , representing cooperativity, were determined using the linear Hill plot (with the logarithm of the free ligand fraction concentration as the independent variable) (Figure 10). Changes in the high-affinity binding of LOS and GLP to non-glycated and glycated albumin in binary and ternary systems, based on K a , the number of LOS and GLP molecules bound to one mole of the macromolecule at a specific binding site ( n ), as well as Hill's coefficient of cooperativity, are summarized in Table 3 and Table 4, respectively (λex = 275 nm, λex = 295 nm).
The Scatchard model of ligand-protein interactions postulates that the protein molecule possesses a finite number of specific binding sites for ligands. In this case, the Scatchard dependence r [ L f ] = f ( r ) is linear and intersects the x-axis of the coordinate system (the r-axis). The linear Scatchard plots for the complexes LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC (Figure 8a), GLP-gHSAGLC, GLP-gHSAFRC (Figure 8b), LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst (Figure 8c) and GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst (Figure 8d) at λex = 275 nm (Figure 8) and λex = 295 nm (Figure S4, Supplementary Materials) indicate the existence of one class of equivalent, independent binding sites for LOS and GLP in both non-modified and glycated albumin structures (or a single binding site), characterized by the same association constant K a ​. A non-linear Scatchard dependence resembling a hyperbola was observed for the GLP-HSA complex excited at λex = 275 nm (Figure 8b) and λex = 295 nm (Figure S4b, Supplementary Materials). This phenomenon may result from the presence of more than one class of ligand-binding sites within the albumin structure (heterogeneous binding), the non-specific nature of GLP binding to HSA, and/or negative cooperativity, where the binding of the drug at one site reduces its affinity for the remaining binding sites on the macromolecule. In contrast, for the LOS-gHSAFRC-GLPconst complex excited at λex = 295 nm (Figure S4c, Supplementary Materials), a "cone-shaped" Scatchard plot was obtained, which may indicate positive cooperativity or instability of losartan. Assuming the existence of two classes of binding sites, the binding parameters for GLP-HSA and LOS-gHSAFRC-GLPconst were determined by non-linear regression using the Levenberg-Marquardt algorithm (Table 3 and Table 4).
Figure 9 illustrates the linear course of the Klotz dependence 1 r = f ( 1 L f ) for the binary (Figure 9a and b) and ternary systems (Figure 9c and d) at λex = 275 nm, indicating the binding of ligands to albumins within a single class of binding sites. Notably, for the system LOS-gHSAFRC-GLPconst at λex = 295 nm, a non-linear course of the Klotz dependence was observed (Figure S5, Supplementary Materials).
In the first class of binding sites, the association constants K a ​ determined from the linear Scatchard and Klotz dependencies for the LOS-gHSAGLC and LOS-gHSAFRC complexes when excited at λex = 275 nm and λex = 295 nm are lower than those for the LOS-HSA complex (Table 3). A comparable trend was noted in the ternary system, where the K a ​ are lower for the complexes with glycated (LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst) compared to non-modified albumin (LOS-HSA-GLPconst). This suggests that albumin glycation reduces the stability of the formed complex for both the excited Trp-214 and the Tyr residues. Losartan has the lowest affinity for fructose-glycated protein (gHSAFRC). Moreover, the presence of an additional drug, i.e., GLP, in the LOS-albumin system weakens the binding of LOS to the macromolecules, as evidenced by a decrease in K a ​ (Table 3). For the LOS-gHSAFRC-GLPconst complex excited at λex = 295 nm, the non-linear course of the Klotz plot made it impossible to determine the binding parameters (Figure S5).
The K a constants, determined by linear regression from the dependencies on the Klotz and the Scatchard equations, as well as based on binding isotherms, are significantly higher for the GLP-HSA compared to the GLP-gHSAGLC and GLP-gHSAFRC complex (Table 4). This suggests that glipizide has a greater affinity for non-modified than glycated albumin, forming a more stable complex. These findings align with previous studies by Koyama et al. [30], which used fluorescence quenching techniques to demonstrate that the binding capacity of hypoglycemic drugs to glycated albumin (G-HSA) was significantly lower than to non-modified HSA. Moreover, Wiglusz et al. [31] demonstrated that gliclazide, a popular hypoglycemic drug, binds more weakly to glycated albumin than its native form. These results confirm that glycation alters the protein structure and drug-binding capacity. Furthermore, Chume et al. [32] confirmed that glycation of albumin decreases its binding capacity for hypoglycemic drugs, which has profound implications for the pharmacokinetics and pharmacodynamics of these drugs in diabetic patients. Conversely, for the ternary system, a higher K a was determined for GLP-gHSAGLC-LOSconst compared to GLP-HSA-LOSconst and GLP-gHSAFRC-LOSconst, indicating that glucose glycation increases the stability of the formed GLP-albumin-LOSconst complex. Furthermore, the presence of LOS in the GLP-albumin complex generally weakens the binding of GLP to HSA and gHSAFRC, as reflected in a decrease in K a (Table 4). However, the presence of LOS does not significantly affect the K a value in the complex with albumin glycated by glucose at λex = 275 nm ( K a (GLP-gHSAGLC) ≈ K a (GLP-gHSAGLC-LOSconst)).
In addition, glipizide at a 5:1 GLP:albumin molar ratio has a higher affinity for non-glycated and glycated protein than losartan at a 10:1 LOS:albumin molar ratio. This effect indicates that the transfer of energy from albumin fluorophores (Trp-214 and Tyr residues) to GLP is more efficient than to LOS in both binary (ligand-albumin) and ternary (in the presence of an additional drug at a 1:1 molar ratio, ligand-albumin-ligandconst) complexes. The number of binding sites n close to one indicates the existence of a single specific binding site for LOS and GLP in non-modified and glycated molecules (Table 3 and Table 4).
To determine whether the binding of LOS and GLP to albumins affects the affinity of the ligand for other binding sites within the macromolecule, Hill’s coefficient ( n H ) for cooperativity was calculated based on the linear Hill plot. Figure 10 shows the linear Hill dependence l o g r 1 r = f l o g [ L f ] in the binary LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC (Figure 10a), GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC (Figure 10b), as well as the ternary systems LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst (Figure 10c) and GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst (Figure 10d) at λex = 275 nm.
For the LOS-HSA (Table 3) and the GLP-HSA complex (Table 4), the Hill coefficient values were found to be less than one ( n H < 1 ) at both excitation wavelengths, indicating negative cooperativity. This implies that binding one LOS or GLP molecule at a binding site decreases the affinity for subsequent ligand binding at other sites on non-glycated albumin [33]. Conversely, for the LOS-gHSAFRC-GLPconst complex (Table 3), the Hill coefficient greater than one was observed ( n H > 1 ), suggesting positive cooperativity. Here, the binding of one LOS molecule facilitates the binding affinity for additional molecules within the LOS-gHSAFRC-GLPconst complex when excited at 295 nm. For the remaining systems, the Hill coefficient was approximately one ( n H   ≈ 1), indicating non-cooperative binding of LOS and GLP to the macromolecules, where the binding of one ligand molecule does not affect the binding affinity of subsequent molecules.

2.3. Investigating Ligand Interactions: Spectrophotometric Analysis of Losartan and Glipizide

There are numerous possibilities for mutual interactions between different pharmaceuticals. Some of these interactions are well-documented and thus can be easily avoided during treatment. However, other medicine interactions are often uncovered only after investigating the underlying causes of treatment failure. Understanding these interactions is crucial, as it can significantly optimize therapeutic outcomes, potentially leading to better patient care and minimizing adverse effects. In this study, in addition to spectrofluorimetry, spectrophotometric measurements were conducted to verify the hypothesis that GLP and LOS can interact not only with non-glycated (HSA) and glycated albumin (gHSAGLC, gHSAFRC) (as discussed in Chapter 2.2.) but also with each other.
Figure 11 shows the absorption spectra of GLP, LOS, and the drug complex (GLP+LOS), from which the absorbance values at selected wavelengths were read. The results are presented in Table 5.
If the absorbance of a mixture of two substances deviates from the mathematical sum of their individual absorbances, it may indicate potential mutual interactions, as suggested by Ren et al. [34]. By observing differences in the absorbance values of GLP and LOS in their combined mixture (GLP+LOS), compared to the expected mathematical sum of their absorbances (Figure 11, Table 5), it can be inferred that GLP and LOS interact with each other. These interactions emphasize the importance of closely monitoring patients' co-administered LOS and GLP, mainly focusing on blood glucose levels, blood pressure, and renal function to ensure safe and effective therapy.

2.4. Spectropolarimetric Analysis of Glycation and Losartan Influence on Macromolecule Secondary Structure

Circular dichroism (CD) spectroscopy was used to evaluate the impact of the glycation process and the presence of losartan (LOS) on the secondary structure of human serum albumin (Figure 12). CD spectroscopy is a valuable analytical technique for assessing the secondary structure of chiral molecules, particularly proteins. It can monitor conformational protein changes, such as folding/unfolding, ligand binding, and protein-protein interactions [35]. CD measurements in the far-UV region can provide quantitative assessments of secondary structure, which can be compared to findings from X-ray crystallography or NMR studies [36].
Table 6 and Table 7 present the value of non-glycated and glycated albumin mean residue ellipticity [ θ ] m r w and the percentage content (%) of albumin secondary structure elements in the sample without (HSA, gHSAGLC, gHSAFRC) and in the presence of losartan at molar ratio of LOS:albumin 10:1 (LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC).
According to the data presented in Table 6 and Table 7, it can be inferred that both non-glycated and glycated albumin primarily display an α-helical structure. The CD spectrum of HSA is characterized by a strong double minimum at λmin = 209.2 nm and λmin = 221.2 nm, which shifts slightly towards shorter wavelengths due to albumin glycation (Figure 12a, Table 6). Absorption in the region below λ = 240 nm is primarily attributed to the peptide bond, featuring a weak but broad n → π* transition centred around λ = 220 nm and a more intense π → π* transition near λ = 190 nm [36]. The reduction in mean residue ellipticity [ θ ] m r w and CD band intensity observed, especially in glycated gHSAFRC compared to non-glycated HSA (Figure 12a, Table 6), may indicate a decrease in α-helix content (gHSAFRC 16.6%) and an increase in β-sheet content of albumin after glycation by fructose (gHSAFRC 6.5%) (Table 7). Mou et al. observed significant changes in the secondary structure of bovine serum albumin (BSA) after glycation by ribose (RBSA). They indicated that an increase in β-sheet content in RBSA is pivotal for protein aggregation [37]. On the other hand, some authors have proposed that glycation may induce aggregation not by unfolding but through overall stabilization of the macromolecule, enhancing protein stability and prolonging its lifespan [38].
The formation of LOS-albumin complexes did not substantially impact the wavelength at which the spectrum reaches its minimum or the mean residue ellipticity values (Table 6). As demonstrated in Table 7, the binding of LOS to HSA and gHSAGLC did not lead to significant alterations in the macromolecule's secondary structure beyond 2%. Similarly, as in this work, Żurawska-Płaksej et al. observed only slight changes in the secondary structure of non-glycated and glycated BSA upon binding with gliclazide (GLICL). The authors emphasized that the decrease in α-helix content indicates a certain degree of structural unfolding, suggesting that GLICL is a weak modifier of BSA's secondary structure [39]. However, in the presented study, the α-helix content of gHSAFRC increased from 20% to 29.9% upon interaction with LOS (Table 7). This result may indicate that LOS stabilizes the secondary structure of the glycated by fructose protein. This stabilization could result from forming new hydrogen bonds or other interactions between the ligand and albumin, leading to more significant structural organization and increased α-helix content. Based on the DSSP (Dictionary of Secondary Structure of Proteins) method, Moeinpour et al. observed that LOS subtly impacts hydrogen bonds and, consequently, the secondary structure of HSA [40]. It should be emphasized that studies using CD spectroscopy to investigate the secondary structure of proteins after glycation are inconclusive. Some researchers have noted glucose concentration-dependent changes in CD spectra, while others have observed partial denaturation and structural disintegration [41]. The results presented in this study indicate that various sugars, as glycation inducers, can affect the secondary structure of human serum albumin differently.

3. Materials and Methods

3.1. Chemicals and Reagents

ImmunO Human serum albumin, fraction V, was purchased from MP Biomedicals LLC (Illkirch, France) and used without further purification; glipizide (GLP), losartan (LOS), sodium azide (NaN3) and dimethyl sulfoxide (DMSO) were provided by Sigma-Aldrich Chemical Co. (Darmstadt, Germany); D(-)-fructose (FRC), D(+)-glucose (GLC) were obtained from POCH S.A. (Gliwice, Poland); di-Potassium hydrogen phosphate pure p.a. (K2HPO4) and sodium dihydrogen phosphate dehydrate (NaH2PO4 × 2H2O) were from Eurochem BGD Sp. z o.o. (Tarnów, Poland). All chemicals and reagents were of the highest analytical grade.

3.2. Methods

3.2.1. Sample Preparation

HSA Glycation: Before the in vitro glycation of human serum albumin (HSA), all glassware and spatulas were sterilized to prevent bacterial contamination. Glycated albumins (gHSAGLC and gHSAFRC) were prepared by exposing HSA solutions (5 × 10−6 mol∙L−1) to D(+)-glucose (GLC) (0.05 mol∙L-1) and D(-)-fructose (FRC) (0.05 mol∙L-1) in a phosphate buffer (0.05 mol∙L-1) preserved with sodium azide (0.015 mol∙L-1) for 21 days incubation at a temperature of t = 37°C. A control sample (HSA) was prepared in the same manner but without the addition of reducing sugars. After the incubation period, the non-glycated HSA and glycated albumins were extensively dialyzed against phosphate buffer (pH = 7.4 ± 0.1) for 24 hours to remove the excess unbound GLC and FRC, then passed through a sterile Millex-GP syringe filter with 0.2 μm pores. The pH of the buffer solution, HSA, gHSAGLC and gHSAFRC was confirmed using a pH meter (FEP20 Mettler Toledo, Columbus, Ohio, USA). The absorbance ratio of HSA, gHSAGLC and gHSAFRC at λ = 255 nm and λ = 280 nm was less than 0.5, indicating the purity of the prepared albumin solutions.
Investigating the Interaction of Losartan (LOS) and Glipizide (GLP) with Non-glycated and Glycated Human Serum Albumins in Binary and Ternary Complexes: A quantitative analysis of the competition between LOS and GLP for the binding site in HSA, gHSAGLC and gHSAFRC was conducted using fluorimetric titration. To obtain the binary complexes of LOS and GLP with non-glycated and glycated albumins (LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC, and GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC), the albumin solutions (5 × 10−6 mol∙L−1) were titrated directly in the cuvette by adding increasing aliquots of LOS (5 × 10−3 mol∙L−1) and GLP (2.5 × 10−3 mol∙L−1) using a Hamilton syringe. The concentration range for LOS was from 5 × 10−6 mol∙L−1 to 5 × 10−5 mol∙L−1, and for GLP, it was from 2.5 × 10−6 mol∙L−1 to 2.5 × 10−5 mol∙L−1. To obtain the ternary complexes LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst, GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, and GLP-gHSAFRC-LOSconst, the albumin solution (5 × 10−6 mol∙L−1) in the presence of GLP (5 × 10−6 mol·L−1) or LOS (5 × 10−6 mol·L−1) (molar ratio drug:albumin 1:1) was titrated in the cuvette by adding ten aliquots of LOS (5 × 10−3 mol∙L−1) or GLP (2.5 × 10−3 mol∙L−1), respectively. This procedure was conducted directly before fluorescence measurements. The LOS and GLP stock solutions were meticulously prepared by dissolving the appropriate amounts in distilled water and DMSO (ensuring DMSO did not exceed 1% v/v in the final concentration), respectively.
Investigating Ligand Interactions–Spectrophotometric Analysis of LOS and GLP: The solutions of LOS and GLP at a concentration of 2.5 × 10−5 mol∙L−1, as well as the drug mixture (GLP+LOS; GLP:LOS molar ratio 1:1), were prepared in phosphate buffer (pH = 7.4 ± 0.1, 0.05 mol∙L-1), by diluting the stock solutions of the drugs (2.5 × 10−3 mol∙L−1 ).
Spectropolarimetric Analysis of Glycation and LOS Influence on Macromolecule Secondary Structure: In this study, the samples (HSA, gHSAGLC, and gHSAFRC at a concentration of 5 × 10−6 mol·L−1 each, as well as the LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC complexes, where the molar ratio of LOS to albumin was 10:1) were prepared according to the procedure described above.

3.2.2. Fluorescence, UV-Vis and Dichroism (CD) Spectra Measurements

The samples’ fluorescence spectra were measured at t = 37°C using a JASCO FP-6500 spectrofluorimeter (Hachioji, Tokyo, Japan) equipped with a Peltier thermostat and standard quartz cells. Excitation at λex = 335 nm (λem = 350–500 nm) and λex = 485 nm (λem = 500–580 nm) was used to measure the fluorescence of Advanced Glycation End-products (AGEs) in non-glycated (HSA) and glycated human serum albumin (gHSAGLC, gHSAFRC).
To excite the albumin fluorophores (Tyr and Trp-214 residues) in the binary (LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC, GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC) and ternary systems (LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst, GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, and GLP-gHSAFRC-LOSconst), excitation wavelengths of λex = 275 nm (excites Tyr and Trp-214 residues, λem = 285–400 nm) and λex = 295 nm (excites Trp-214 residue, λem = 305–400 nm) were used. Finally, using JASCO software (Spectra Manager), the light scattering spectrum of the buffer was subtracted from all fluorescence spectra.
Due to the inner filter effect resulting from the presence of the drugs, the recorded fluorescence of HSA, gHSAGLC, gHSAFRC in the binary and ternary systems was corrected using Equation (1) [42]:
F c o r = F o b s · e A b s e x + A b s e m 2
where: F c o r and F o b s are the corrected and observed fluorescence intensities, respectively; and A b s e x and A b s e m are the absorbance at the excitation and emission wavelengths, respectively.
The samples' absorbance measurements were recorded using a model V-760 JASCO spectrophotometer (Easton, Maryland, USA) equipped with a thermostat bath, using quartz cuvettes of dimensions 1.0 cm × 1.0 cm × 4.0 cm. The apparatus has a wavelength correction error of ± 0.3 nm and a photometric correction error of ± 0.002 Abs at 0.5 Abs.
The absorption spectra of GLP and LOS at a concentration of 2.5 × 10−5 mol∙L−1, as well as the GLP+LOS system at GLP:LOS 1:1 (v/v) molar ratio, were determined in the wavelength range of λ = 235–300 nm at t = 37°C.
Far-UV CD spectra of HSA, gHSAGLC, gHSAFRC and LOS-HSA, LOS-gHSAGLC, and LOS-gHSAFRC complexes were recorded using a JASCO model J-1500 CD spectropolarimeter (Hachioji, Tokyo, Japan) equipped with a thermostatic Peltier cell holder (accuracy t = ± 0.05°C). All spectra were measured in a 0.1 cm path length quartz cuvette and scanned from λ = 200–250 nm at wavelength intervals of 0.2 nm, with a bandwidth set at 2.0 nm and D.I.T. of 4 seconds. CD intensity is expressed as mean residue ellipticity at wavelength λ ( [ θ ] m r w ) (deg·cm2·dmol−1) according to Equation (2) [36]:
θ m r w = M R W · θ λ 10 · d · c
where: M R W is the Mean Residue Weight ( M R W H S A = 113.7 Da); θ λ is the observed ellipticity at wavelength λ (deg); d is the optical path–length (cm); c is the protein concentration (g·cm−3).
The content of the samples' secondary structure elements was calculated using the Secondary Structure Estimation program with Yang's Reference model.
The fluorescence, absorption, and Far-UV CD spectra presented in this study were corrected by smoothing using the Savitzky and Golay method with a convolution width of 15, using the Spectra Analysis program (version 1.53.07, JASCO, Easton, Maryland, USA). Linear regression was performed by fitting the experimental data to the corresponding equation using Origin version 8.5 software (Northampton, MA, USA).
Based on the calculated fluorescence emission intensities, the quenching curves ( F F 0 vs. drug:albumin molar ratio, where: F , F 0 are the fluorescence intensities in the presence and absence of the quencher, respectively) of non-glycated and glycated human serum albumin in the presence of losartan (LOS) or glipizide (GLP) (binary system: LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC and GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC) or in the presence of both drugs (ternary system: LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst and GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst) were plotted.
The fluorescence quenching mechanism of HSA, gHSAGLC and gHSAFRC in the absence or presence of LOS and GLP in the binary and ternary systems was analyzed based on the Stern-Volmer equation (Equation (3)) [27]:
F 0 F = 1 + k q τ 0 · Q = 1 + K S V · [ Q ]
where: k q is the bimolecular quenching rate constant (L∙mol−1∙s−1), k q = K S V τ 0 ; τ 0 is the average fluorescence lifetime of albumin without a quencher, τ 0 = 6.0 × 10−9 s [26]; K S V is the Stern-Volmer constant (L∙mol−1); Q is the concentration of the quencher (mol∙L−1).
The association constant ( K a ) and the number of binding sites classes ( n ) in the ligand-albumin or ligand-albumin-ligandconst complexes were determined using the Scatchard (Equation (4)) [43] and Klotz (Equation (5)) equations [44]:
r [ L f ] = n · K a K a · r
1 r = 1 n + 1 n · K a · [ L f ]
where: r = [ L b ] [ P ] is the number of ligand moles bound to one mole of protein; L b and L f are the bound and unbound drug concentrations, respectively and P is the total protein concentration (mol∙L−1).
For two classes of binding sites in albumin structure (in this study GLP-HSA and LOS-gHSAFRC-GLPconst complexes), the binding isotherms were drawn using non-linear regression analysis according to Equation (6) and the association constants ( K a 1 ,    K a 2 ) and the number of binding sites ( n 1 ,   n 2 ) were calculated [45]:
r = n 1 · K a 1 · L f 1 + K a 1 · L f + n 2 · K a 2 · L f 1 + K a 2 · L f
Hill’s coefficient n H was determined on the basis of the Hill method (Equation (6)) [46]:
l o g r 1 r = n H · l o g [ L f ] + l o g K a

4. Conclusions

The main goal of this project was to analyze the interactions of losartan (LOS) and glipizide (GLP) with non-glycated (HSA) and glycated human serum albumin (gHSAGLC and gHSAFRC) and to investigate their mutual competition in the binding sites of the macromolecule using multiple spectroscopic techniques.
The analysis of the emission fluorescence spectra of glycation products (AGEs) indicated that fructose (FRC) is a more effective glycation agent for HSA than glucose (GLC). This conclusion is supported by the observation that glycation in the presence of FRC leads to a faster and more efficient Amadori rearrangement. Glycation induces conformational changes in the albumin structure, particularly altering the microenvironment around crucial amino acid residues (Trp-214 and Tyr), thus influencing their accessibility to quenchers. The results showed that LOS and GLP have a higher affinity for non-glycated HSA than glycated gHSAGLC and gHSAFRC, forming a more stable complex. Additionally, LOS and GLP were found to interact nonspecifically with the hydrophobic fragments of the surface of albumins in binary (ligand-albumin) and ternary systems (ligand-albumin-ligandconst) and specifically saturate the binding sites within the protein molecule. An additional drug (GLP in the LOS-albumin complex or LOS in the GLP-albumin complex) complicates the interaction, likely leading to competitive binding or displacement of the initially bound drug in both non- and glycated albumins. Analysis of the CD spectra revealed that GLP and LOS interact with each other. This finding emphasizes the importance of closely monitoring patients' co-administered these drugs, focusing on blood glucose levels, blood pressure, and renal function to ensure safe and effective therapy.
In conclusion, the significant impact of glycation on the drug-binding capacity of albumin, as revealed by this study, has profound implications for patient care. Particularly for diabetic patients, the altered binding properties of glycated albumin could potentially compromise the efficacy and safety of drug therapy. Therefore, the need for careful monitoring and potentially adjusted dosing regimens is urgent to ensure optimal therapeutic outcomes. Further clinical studies are imperative to develop comprehensive guidelines for the concurrent use of LOS and GLP in polypharmacotherapy.

Supplementary Materials

The following supporting information can be downloaded at: Preprints.org, Figure S1: Quenching fluorescence of albumin non-glycated (HSA, ◆) and glycated (gHSAGLC, ◊; gHSAFRC, ◆) containing 5 × 10−6 mol∙L−1 to 5 × 10−5 mol∙L−1 concentrations of LOS (a, b) and 2.5 × 10−6 mol∙L−1 to 2.5 × 10−5 mol∙L−1 concentrations of GLP (c, d). Albumin concentration: 5 × 10−6 mol∙L−1; λex = 275 nm (a, c) and λex = 295 nm (b, d); error bars are smaller than the symbols; Figure S2: The Stern-Volmer curves for the binary (a) LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC; (b) GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC and ternary systems (c) LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst; (d) GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst; λex = 295 nm; error bars are smaller than the symbols used in the plots; Figure S3: Binding isotherms of HSA, gHSAGLC and gHSAFRC at 5 × 10−6 mol∙L−1 concentration with LOS at 5 × 10−6 mol∙L−1 to 5 × 10−5 mol∙L−1 and GLP at 2.5 × 10−6 mol∙L−1 to 2.5 × 10−5 mol∙L−1 concentrations in the binary (a) LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC; (b) GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC and ternary systems (c) LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst; with GLP at 5 × 10−6 mol∙L−1 concentration, (d) GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst with LOS at 5 × 10−6 mol∙L−1 concentration, λex = 295 nm; error bars are smaller than the symbols used in the plots; Figure S4: Scatchard plots for the binary (a) LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC; (b) GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC and ternary systems (c) LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst; (d) GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst; λex = 295 nm; error bars are smaller than the symbols used in the plots; Figure S5: Klotz curves for the binary (a) LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC; (b) GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC and ternary systems (c) LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst; (d) GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst; λex = 295 nm; error bars are smaller than the symbols used in the plots; Figure S6: Hill plots for the binary (a) LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC; (b) GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC and ternary systems (c) LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst; (d) GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst; λex = 295 nm; error bars are smaller than the symbols used in the plots; Table S1: The percentage (%) of fluorescence quenching of non-glycated (HSA) and glycated albumin (gHSAGLC, gHSAFRC) in the presence of losartan (LOS) and glipizide (GLP) with increasing concentration; λex = 275 nm and λex = 295 nm.

Author Contributions

Conceptualization, A.S.; methodology, A.S.; software, A.S.; validation, A.S.; formal analysis, A.S.; investigation, A.S.; resources, A.S.; data curation, A.S.; writing—original draft preparation, A.S.; writing—review and editing, A.S.; visualization, A.S.; supervision, A.S.; project administration, A.S.; funding acquisition, A.S. The author has read and agreed to the published version of the manuscript.

Funding

This research was funded by the Medical University of Silesia, Katowice, Poland (Grant No. PCN-2-012/K/1/F and PCN-2-013/K/2/F).

Institutional Review Board Statement

Not applicable.

Informed Consent Statement

Not applicable.

Data Availability Statement

The data underlying the findings of this study are accessible upon reasonable request to the author.

Conflicts of Interest

The author declares no conflicts of interest. The funders had no role in the design of the study; in the collection, analyses, or interpretation of data; in the writing of the manuscript; or in the decision to publish the results.

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Figure 1. Chemical structure of (a) losartan (LOS) and (b) glipizide (GLP). The structural formulas of LOS and GLP were rendered using the ChemSketch ver. 12.1.0.31258 program.
Figure 1. Chemical structure of (a) losartan (LOS) and (b) glipizide (GLP). The structural formulas of LOS and GLP were rendered using the ChemSketch ver. 12.1.0.31258 program.
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Figure 2. Emission fluorescence spectra of AGEs present in HSA and formed in gHSAGLC and gHSAFRC excited at (a) λex = 335 nm and (b) λex = 485 nm; protein concentration is 5 × 10⁻⁶ mol∙L⁻¹.
Figure 2. Emission fluorescence spectra of AGEs present in HSA and formed in gHSAGLC and gHSAFRC excited at (a) λex = 335 nm and (b) λex = 485 nm; protein concentration is 5 × 10⁻⁶ mol∙L⁻¹.
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Figure 3. Quenching fluorescence of HSA (a, d), gHSAGLC (b, e) and gHSAFRC (c, f) containing 5 × 10−6 mol∙L−1 to 5 × 10−5 mol∙L−1 concentrations of LOS (ac) and 2.5 × 10−6 mol∙L−1 to 2.5 × 10−5 mol∙L−1 concentrations of GLP (df). Albumin concentration: 5 × 10−6 mol∙L−1; λex = 275 nm (◆) and λex = 295 nm (◊); error bars are smaller than the symbols.
Figure 3. Quenching fluorescence of HSA (a, d), gHSAGLC (b, e) and gHSAFRC (c, f) containing 5 × 10−6 mol∙L−1 to 5 × 10−5 mol∙L−1 concentrations of LOS (ac) and 2.5 × 10−6 mol∙L−1 to 2.5 × 10−5 mol∙L−1 concentrations of GLP (df). Albumin concentration: 5 × 10−6 mol∙L−1; λex = 275 nm (◆) and λex = 295 nm (◊); error bars are smaller than the symbols.
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Figure 4. Quenching fluorescence of HSA (a, b), gHSAGLC (c, d) and gHSAFRC (e, f) by LOS and in the presence of GLP at 5 × 10−6 mol∙L−1 concentration. LOS concentration varied from 5 × 10−6 mol∙L−1 to 5 × 10−5 mol∙L−1. The proteins concentration: 5 × 10−6 mol∙L−1; λex = 275 nm (a, c, e) and λex = 295 nm (b, d, f); error bars, indicating the standard deviation, are smaller than the symbols used in the plots.
Figure 4. Quenching fluorescence of HSA (a, b), gHSAGLC (c, d) and gHSAFRC (e, f) by LOS and in the presence of GLP at 5 × 10−6 mol∙L−1 concentration. LOS concentration varied from 5 × 10−6 mol∙L−1 to 5 × 10−5 mol∙L−1. The proteins concentration: 5 × 10−6 mol∙L−1; λex = 275 nm (a, c, e) and λex = 295 nm (b, d, f); error bars, indicating the standard deviation, are smaller than the symbols used in the plots.
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Figure 5. Quenching fluorescence of HSA (a, b), gHSAGLC (c, d) and gHSAFRC (e, f) by GLP and in the presence of LOS at 5 × 10−6 mol∙L−1 concentration. GLP concentration varied from 2.5 × 10−6 mol∙L−1 to 2.5 × 10−5 mol∙L−1. Protein concentration: 5 × 10−6 mol∙L−1; λex = 275 nm (a, c, e) and λex = 295 nm (b, d, f); error bars, indicating the standard deviation, are smaller than the symbols used in the plots.
Figure 5. Quenching fluorescence of HSA (a, b), gHSAGLC (c, d) and gHSAFRC (e, f) by GLP and in the presence of LOS at 5 × 10−6 mol∙L−1 concentration. GLP concentration varied from 2.5 × 10−6 mol∙L−1 to 2.5 × 10−5 mol∙L−1. Protein concentration: 5 × 10−6 mol∙L−1; λex = 275 nm (a, c, e) and λex = 295 nm (b, d, f); error bars, indicating the standard deviation, are smaller than the symbols used in the plots.
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Figure 6. The Stern-Volmer curves for the binary (a) LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC; (b) GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC and ternary systems (c) LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst; (d) GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst; λex = 275 nm; error bars are smaller than the symbols used in the plots.
Figure 6. The Stern-Volmer curves for the binary (a) LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC; (b) GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC and ternary systems (c) LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst; (d) GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst; λex = 275 nm; error bars are smaller than the symbols used in the plots.
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Figure 7. Binding isotherms of HSA, gHSAGLC and gHSAFRC at 5 × 10−6 mol∙L−1 concentration with LOS at 5 × 10−6 mol∙L−1 to 5 × 10−5 mol∙L−1 and GLP at 2.5 × 10−6 mol∙L−1 to 2.5 × 10−5 mol∙L−1 concentrations in the binary (a) LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC; (b) GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC and ternary systems (c) LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst; with GLP at 5 × 10−6 mol∙L−1 concentration, (d) GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst with LOS at 5 × 10−6 mol∙L−1 concentration, λex = 275 nm; error bars are smaller than the symbols used in the plots.
Figure 7. Binding isotherms of HSA, gHSAGLC and gHSAFRC at 5 × 10−6 mol∙L−1 concentration with LOS at 5 × 10−6 mol∙L−1 to 5 × 10−5 mol∙L−1 and GLP at 2.5 × 10−6 mol∙L−1 to 2.5 × 10−5 mol∙L−1 concentrations in the binary (a) LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC; (b) GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC and ternary systems (c) LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst; with GLP at 5 × 10−6 mol∙L−1 concentration, (d) GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst with LOS at 5 × 10−6 mol∙L−1 concentration, λex = 275 nm; error bars are smaller than the symbols used in the plots.
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Figure 8. Scatchard plots for the binary (a) LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC; (b) GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC and ternary systems (c) LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst; (d) GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst; λex = 275 nm; error bars are smaller than the symbols used in the plots.
Figure 8. Scatchard plots for the binary (a) LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC; (b) GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC and ternary systems (c) LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst; (d) GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst; λex = 275 nm; error bars are smaller than the symbols used in the plots.
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Figure 9. Klotz curves for the binary (a) LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC; (b) GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC and ternary systems (c) LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst; (d) GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst; λex = 275 nm; error bars are smaller than the symbols used in the plots.
Figure 9. Klotz curves for the binary (a) LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC; (b) GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC and ternary systems (c) LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst; (d) GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst; λex = 275 nm; error bars are smaller than the symbols used in the plots.
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Figure 10. Hill plots for the binary (a) LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC; (b) GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC and ternary systems (c) LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst; (d) GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst; λex = 275 nm; error bars are smaller than the symbols used in the plots.
Figure 10. Hill plots for the binary (a) LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC; (b) GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC and ternary systems (c) LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst; (d) GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst; λex = 275 nm; error bars are smaller than the symbols used in the plots.
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Figure 11. The absorption spectra of GLP, LOS and the drugs mixture (GLP+LOS); drug concentration is 2.5 × 10⁻5 mol∙L⁻¹; the GLP to LOS molar ratio is 1:1; t = 37°C.
Figure 11. The absorption spectra of GLP, LOS and the drugs mixture (GLP+LOS); drug concentration is 2.5 × 10⁻5 mol∙L⁻¹; the GLP to LOS molar ratio is 1:1; t = 37°C.
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Figure 12. Far-UV CD spectra of (a) non-glycated (HSA) and glycated (gHSAGLC, gHSAFRC) human serum albumin; (b) HSA and LOS-HSA; (c) gHSAGLC and LOS-gHSAGLC; (d) gHSAFRC and LOS-gHSAFRC; protein concentration equals 5 × 10−6 mol∙L−1; the LOS to albumin molar ratio is 10:1; t = 37°C.
Figure 12. Far-UV CD spectra of (a) non-glycated (HSA) and glycated (gHSAGLC, gHSAFRC) human serum albumin; (b) HSA and LOS-HSA; (c) gHSAGLC and LOS-gHSAGLC; (d) gHSAFRC and LOS-gHSAFRC; protein concentration equals 5 × 10−6 mol∙L−1; the LOS to albumin molar ratio is 10:1; t = 37°C.
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Table 1. Stern-Volmer constants K S V (L∙mol−1), fractional accessible albumin fluorescence f a , and the bimolecular quenching rate constant k q (L∙mol−1∙s−1) calculated for LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC and LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst; λex = 275 nm and λex = 295 nm.
Table 1. Stern-Volmer constants K S V (L∙mol−1), fractional accessible albumin fluorescence f a , and the bimolecular quenching rate constant k q (L∙mol−1∙s−1) calculated for LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC and LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst; λex = 275 nm and λex = 295 nm.
λex = 275 nm K S V ± RSD *) × 104 (L∙mol−1) f a ± RSD *) a)  k q ± RSD *) × 1012 (L∙mol−1∙s−1)
LOS-HSA 1.92 ± 0.04 0.96 ± 0.01 3.20 ± 0.07
LOS-gHSAGLC 1.42 ± 0.01 0.99 2.36 ± 0.02
LOS-gHSAFRC 0.84 ± 0.01 1.00 1.40 ± 0.01
LOS-HSA-GLPconst 2.40 ± 0.02 1.01 4.00 ± 0.03
LOS-gHSAGLC-GLPconst 2.16 ± 0.01 1.00 3.61 ± 0.01
LOS-gHSAFRC-GLPconst 1.66 ± 0.01 1.00 2.77 ± 0.02
λex = 295 nm K S V  ± RSD *) × 104 (L∙mol−1) f a   ± RSD *) a)  k q   ± RSD *) × 1012 (L∙mol−1∙s−1)
LOS-HSA 1.64 ± 0.05 0.96 ± 0.02 2.71 ± 0.09
LOS-gHSAGLC 0.99 ± 0.02 0.98 ± 0.01 1.66 ± 0.03
LOS-gHSAFRC 0.40 ± 0.01 1.00 0.66 ± 0.01
LOS-HSA-GLPconst 1.59 ± 0.02 0.99 2.65 ± 0.03
LOS-gHSAGLC-GLPconst 1.24 ± 0.02 1.00 2.07 ± 0.03
LOS-gHSAFRC-GLPconst 0.68 ± 0.01 1.00 1.13 ± 0.02
*) Relative Standard Deviation; a) calculated using: k q = K S V τ 0 , where: τ 0 = 6.0 × 10−9 s [26]—the fluorescence lifetime of albumin in the absence of a quencher.
Table 2. Stern-Volmer constants K S V (L∙mol−1), fractional accessible protein fluorescence f a , and the bimolecular quenching rate constant k q (L∙mol−1∙s−1) calculated for GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC and GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst; λex = 275 nm and λex = 295 nm.
Table 2. Stern-Volmer constants K S V (L∙mol−1), fractional accessible protein fluorescence f a , and the bimolecular quenching rate constant k q (L∙mol−1∙s−1) calculated for GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC and GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst; λex = 275 nm and λex = 295 nm.
λex = 275 nm K S V  ± RSD *) × 104 (L∙mol−1) f a  ± RSD *) a)  k q  ± RSD *) × 1012 (L∙mol−1∙s−1)
GLP-HSA 5.31 ± 0.13 0.93 ± 0.02 8.85 ± 0.20
GLP-gHSAGLC 3.86 ± 0.01 0.99 6.44 ± 0.02
GLP-gHSAFRC 2.54 ± 0.01 1.00 4.23 ± 0.03
GLP-HSA-LOSconst 3.41 ± 0.02 1.01 5.69 ± 0.04
GLP-gHSAGLC-LOSconst 3.73 ± 0.02 0.99 6.21 ± 0.03
GLP-gHSAFRC-LOSconst 2.54 ± 0.02 1.01 4.23 ± 0.04
λex = 295 nm K S V  ± RSD *) × 104 (L∙mol−1) f a  ± RSD *) a)  k q  ± RSD *) × 1012 (L∙mol−1∙s−1)
GLP-HSA 4.05 ± 0.23 0.89 ± 0.02 6.76 ± 0.39
GLP-gHSAGLC 2.34 ± 0.07 0.97 ± 0.01 3.91 ± 0.12
GLP-gHSAFRC 1.09 ± 0.02 0.99 1.82 ± 0.03
GLP-HSA-LOSconst 2.02 ± 0.03 0.98 ± 0.01 3.36 ± 0.06
GLP-gHSAGLC-LOSconst 2.31 ± 0.07 0.97 ± 0.01 3.84 ± 0.12
GLP-gHSAFRC-LOSconst 1.13 ± 0.02 0.99 1.88 ± 0.04
*) Relative Standard Deviation; a) calculated using: k q = K S V τ 0 , where: τ 0 = 6.0 × 10−9 s [26].
Table 3. Association constants K a (L∙mol−1), mean number of LOS molecule bound with one molecule of HSA, gHSAGLC and gHSAFRC  ( n ) , the Hill’s coefficient ( n H ) in the binary (LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC) and ternary system (LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst); λex = 275 nm and λex = 295 nm.
Table 3. Association constants K a (L∙mol−1), mean number of LOS molecule bound with one molecule of HSA, gHSAGLC and gHSAFRC  ( n ) , the Hill’s coefficient ( n H ) in the binary (LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC) and ternary system (LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst); λex = 275 nm and λex = 295 nm.
Scatchard Method Klotz Method Hill Method
λex = 275 nm K a  ± RSD *) × 104 (L∙mol−1) n  ± RSD *) K a  ± RSD *) × 104 (L∙mol−1) n  ± RSD *) n H  ± RSD *)
LOS-HSA 3.76 ± 0.05 0.91 ± 0.02 3.78 ± 0.02 0.91 ± 0.01 0.94
LOS-gHSAGLC 2.31 ± 0.19 1.09 ± 0.12 2.90 ± 0.16 0.93 ± 0.08 1.04 ± 0.02
LOS-gHSAFRC 0.93 ± 0.05 1.12 ± 0.07 1.10 ± 0.07 0.97 ± 0.07 1.02 ± 0.01
LOS-HSA-GLPconst 1.20 ± 0.06 1.11 ± 0.07 1.39 ± 0.09 0.98 ± 0.08 1.02 ± 0.01
LOS-gHSAGLC-GLPconst 1.10 ± 0.01 1.02 ± 0.01 1.13 ± 0.01 0.99 ± 0.01 1.00
LOS-gHSAFRC-GLPconst 0.89 ± 0.04 1.01 ± 0.05 0.93 ± 0.03 0.97 ± 0.04 1.00 ± 0.01
λex = 295 nm K a   ±   RSD   * )   ×   10 4   n L∙mol−1)  ± RSD *) K a  ± RSD *) × 104 (L∙mol−1) n  ± RSD *) n H  ± RSD *)
LOS-HSA 3.61 ± 0.07 0.92 ± 0.03 3.49 ± 0.04 0.94 ± 0.02 0.95 ± 0.01
LOS-gHSAGLC 2.40 ± 0.26 1.12 ± 0.17 3.20 ± 0.23 0.93 ± 0.10 1.06 ± 0.03
LOS-gHSAFRC 0.89 ± 0.07 1.13 ± 0.11 1.06 ± 0.10 0.97 ± 0.10 1.02 ± 0.01
LOS-HSA-GLPconst 1.16 ± 0.02 0.97 ± 0.03 1.16 ± 0.03 0.97 ± 0.03 0.99
LOS-gHSAGLC-GLPconst 0.91 ± 0.08 1.12 ± 0.12 1.09 ± 0.12 0.96 ± 0.12 1.02 ± 0.01
LOS-gHSAFRC-GLPconst a) 0.59 ± 0.01 a) 0.85 ± 0.01 - **) - **) 1.20 ± 0.02
*) Relative Standard Deviation; a) determined by non-linear regression using binding isotherms; **) impossible to determine .
Table 4. Association constants K a (L∙mol−1), mean number of GLP molecule bound with one molecule of HSA, gHSAGLC and gHSAFRC  ( n ) , the Hill’s coefficient ( n H ) in the binary (GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC) and ternary system (GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst); λex = 275 nm and λex = 295 nm.
Table 4. Association constants K a (L∙mol−1), mean number of GLP molecule bound with one molecule of HSA, gHSAGLC and gHSAFRC  ( n ) , the Hill’s coefficient ( n H ) in the binary (GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC) and ternary system (GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst); λex = 275 nm and λex = 295 nm.
Scatchard Method Klotz Method Hill Method
λex = 275 nm K a  ± RSD *) × 104 (L∙mol−1) n  ± RSD *) K a  ± RSD *) × 104 (L∙mol−1) n  ± RSD *) n H  ± RSD *)
GLP-HSA a) 57.84 ± 3.01 a) 0.41 ± 0.02 25.38 ± 0.04 0.85 ± 0.03 0.92 ± 0.03
a) 3.44 ± 0.31 a) 0.97 ± 0.02
GLP-gHSAGLC 6.66 ± 0.30 0.93 ± 0.06 7.48 ± 0.17 0.86 ± 0.03 0.96 ± 0.01
GLP-gHSAFRC 3.27 ± 0.17 1.02 ± 0.07 3.82 ± 0.17 0.91 ± 0.05 1.00 ± 0.01
GLP-HSA-LOSconst 3.96 ± 0.08 0.91 ± 0.02 4.07 ± 0.06 0.89 ± 0.02 0.97
GLP-gHSAGLC-LOSconst 6.58 ± 0.27 0.94 ± 0.06 7.26 ± 0.12 0.88 ± 0.02 0.97 ± 0.01
GLP-gHSAFRC-LOSconst 2.45 ± 0.07 0.89 ± 0.03 2.35 ± 0.09 0.92 ± 0.04 0.98 ± 0.01
λex = 295 nm K a  ± RSD *) × 104 (L∙mol−1) n  ± RSD *) K a  ± RSD *) × 104 (L∙mol−1) n  ± RSD *) n H  ± RSD *)
GLP-HSA a) 112.04 ± 25.01 a) 0.34 ± 0.05 36.45 ± 0.20 0.83 ± 0.03 0.84 ± 0.03
a) 7.52 ± 1.29 a) 0.77 ± 0.02
GLP-gHSAGLC 8.40 ± 0.41 0.93 ± 0.07 9.43 ± 0.11 0.87 ± 0.02 0.96 ± 0.01
GLP-gHSAFRC 2.69 ± 0.19 1.06 ± 0.10 3.23 ± 0.19 0.92 ± 0.07 1.01 ± 0.01
GLP-HSA-LOSconst 5.15 ± 0.22 0.97 ± 0.06 5.77 ± 0.15 0.89 ± 0.03 0.99 ± 0.01
GLP-gHSAGLC-LOSconst 7.30 ± 0.16 0.89 ± 0.03 7.50 ± 0.09 0.88 ± 0.02 0.94
GLP-gHSAFRC-LOSconst 2.92 ± 0.14 0.87 ± 0.05 2.69 ± 0.13 0.93 ± 0.05 0.97 ± 0.01
*) Relative Standard Deviation; a) determined by non-linear regression using binding isotherms.
Table 5. The values of maximum absorbance of GLP, LOS and drugs mixture at the selected wavelengths λ = 235 nm, λ = 253 nm, and λ = 282 nm.
Table 5. The values of maximum absorbance of GLP, LOS and drugs mixture at the selected wavelengths λ = 235 nm, λ = 253 nm, and λ = 282 nm.
λ (nm) Absorbance (a.u.) Mathematic sum of GLP and LOS absorbance
GLP LOS GLP+LOS
235 0.9319 1.9768 2.5215 2.9087
253 0.1545 1.2960 1.4173 1.4505
282 0.2549 0.2456 0.4509 0.5005
Table 6. The values of non-glycated and glycated albumin mean residue ellipticity [ θ ] m r w in the sample without (HSA, gHSAGLC, gHSAFRC) and in the presence of losartan (LOS-HSA, LOS- gHSAGLC, LOS-gHSAFRC).
Table 6. The values of non-glycated and glycated albumin mean residue ellipticity [ θ ] m r w in the sample without (HSA, gHSAGLC, gHSAFRC) and in the presence of losartan (LOS-HSA, LOS- gHSAGLC, LOS-gHSAFRC).
Sample* λmin (nm) [ θ ] m r w (deg·cm2·dmol−1) HT (V)
HSA 209.2 −13,855.23 281.61
221.2 −13,087.41 242.06
gHSAGLC 208.8 −12,324.99 284.85
221.2 −11,529.40 242.88
gHSAFRC 208.6 −11,871.22 286.79
221.2 −10,453.40 243.58
LOS-HSA 209.2 −13,869.50 301.08
221.2 −13,035.94 254.15
LOS-gHSAGLC 208.8 −11,993.66 298.99
221.2 −11,273.80 251.65
LOS-gHSAFRC 208.6 −11,513.06 300.09
221.2 −10,230.25 253.13
*for the remaining complexes (GLP-HSA, GLP-gHSAGLC, GLP-gHSAFRC, GLP-HSA-LOSconst, GLP-gHSAGLC-LOSconst, GLP-gHSAFRC-LOSconst, LOS-HSA-GLPconst, LOS-gHSAGLC-GLPconst, LOS-gHSAFRC-GLPconst), obtaining CD spectra was impossible due to excessively weak signals likely caused by too low a concentration of GLP. This resulted in the sample absorbance exceeding the detector's capacity, leading to off-scale signals – HT (High Tension) readings outside the acceptable range.
Table 7. The percentage content (%) of non-glycated and glycated albumin secondary structure elements in the sample without (HSA, gHSAGLC, gHSAFRC) and in the presence of losartan (LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC) based on the Yang’s Reference model.
Table 7. The percentage content (%) of non-glycated and glycated albumin secondary structure elements in the sample without (HSA, gHSAGLC, gHSAFRC) and in the presence of losartan (LOS-HSA, LOS-gHSAGLC, LOS-gHSAFRC) based on the Yang’s Reference model.
% α-Helix % β-Sheet % Turn % Random
HSA 36.6 10.2 22.6 30.6
gHSAGLC 35.7 11.1 22.4 30.8
gHSAFRC 20.0 16.7 21.6 32.7
LOS-HSA 35.7 8.8 23.9 31.7
LOS-gHSAGLC 35.8 9.7 23.4 31.1
LOS-gHSAFRC 29.9 15.9 21.9 32.4
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