**1. Introduction**

5

Blood flow and circulation inside vessels in vivo are defined by many interconnected parameters, such as blood viscosity, hematocrit, and plasma protein composition, so to properly study them a complex approach is required [1]. There are many methods allowing for in vivo and in vitro measurements of different blood properties [1,2].

The main focus of this study is the aggregation of red blood cells (RBCs), which significantly influences the viscosity of blood [3]. RBC aggregation is the reversible process of the formation of linear and more complex structures of RBCs. It promotes the formation of peripheral cell-poor fluid layer that lowers the hydrodynamic vessel resistance to blood flow [3]. The process of in vitro as well as in vivo RBC aggregation can be described in several ways: by the number of cells aggregating during a given time interval, by how many aggregates are observed, by how fast a couple of RBCs can form a doublet, etc. [3]. These parameters require specialized tools in order to be measured, so they are not used widely in clinical conditions. RBC aggregation depends on many internal and external factors. For example, blood plasma composition, temperature, RBC shapes, and the age, state of health of an individual, and his or her medicine intake determine in part the aggregation parameters of RBCs [3–5].

Many methods can be applied to studying RBCs, including micropipette aspiration [6], etc., but among all methods it would be worth highlighting the optical techniques as far as they have several advantages: non-invasiveness and lack of direct mechanical contact with

**Citation:** Maslianitsyna, A.; Ermolinskiy, P.; Lugovtsov, A.; Pigurenko, A.; Sasonko, M.; Gurfinkel, Y.; Priezzhev, A. Multimodal Diagnostics of Microrheologic Alterations in Blood of Coronary Heart Disease and Diabetic Patients. *Diagnostics* **2021**, *11*, 76. https://doi.org/10.3390/ diagnostics11010076

Received: 4 November 2020 Accepted: 30 December 2020 Published: 6 January 2021

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the cells, the option to study both individual cells and their ensembles, and the possibility of in vivo and in vitro application [4,7]. The last point can pose a challenge in terms of comparing results for these different conditions—in vitro measurements require anticoagulants for stabilizing the blood samples and storing blood during sample preparation, which can influence the measured parameters, whereas in vivo methods allow for measuring a different set of parameters that may be difficult to correlate with those measured in vitro.

The aim of this work was to find correspondence between in vivo and in vitro optical methods by studying patients with cardiovascular and associated pathologies. Understanding the link between RBC aggregation and widespread cardiovascular diseases is vital to create new methods of diagnosis and treatment. In this article, we look at coronary heart disease (CHD) and type 2 diabetes mellitus (T2DM), which are known to have a significant effect on microvasculature [8].

#### **2. Materials and Methods**

*2.1. Patients*

The study enrolled 81 adults, including 25 healthy volunteers and 56 patients with CHD and arterial hypertension (Table 1). The patients with CHD were divided into two groups depending on the presence of T2DM. The first group included 42 CHD patients without T2DM, and second group included 14 CHD patients with T2DM. We did not find any statistically significant differences in the clinical background for these two groups of patients. The study was conducted during the period from July 2015 to July 2020.

**Table 1.** The clinical backgrounds for each group of patients, mean ± standard deviation or number (%).


CHD—coronary heart disease; T2DM—type 2 diabetes mellitus; LV ejection fraction—left ventricular ejection fraction.

> Criteria for exclusion from the study were the following: chronic heart disease insufficiency, heart rhythm and conduction disorders, renal and hepatic insufficiency, type 1 diabetes mellitus, vascular or other pathology of the brain, or oncological diseases in the medical history.

> The study included several procedures for the patients. The measurements of blood pressure and heart rate were conducted for each patient between 8:00 and 8:30 a.m. before their medicine intake on the day following their hospitalization in the cardiological unit. In addition to the standard medical check-up, all patients underwent a non-invasive study of microcirculatory parameters in the nail bed capillaries using the method of digital capillaroscopy. For the in vitro study, the blood was drawn from the patients' cubital veins on an empty stomach, stabilized with EDTA K2 anticoagulant and was used for the experiments within the first three hours.

Twenty-five healthy volunteers (16 males and 9 females) had an average age 27.5 and body mass index (BMI) of 22.1, were non-smokers, and had not taken any medication. These people were divided into two control groups (*n* = 10 (4 males and 6 females) and 15 (12 males and 3 females)) that were studied independently at different time intervals with different parameters measured.

The study design was approved by the local ethics committee of medical research and educational center of M.V. Lomonosov Moscow State University, Moscow, Russia (protocol code: 1/19, date of approval: 18 February 2019). The experiment design took into account the latest recommendations for laboratories made by the international expert team for the standardization of hemorheological methods [9]. The patients and healthy volunteers participating in the research were informed on the purpose of the study and gave written informed consent in accordance with the Declaration of Helsinki.

#### *2.2. Laser Aggregometry Method*

The laser aggregometry method implemented in a microchip stirring type RheoScan aggregometer (RheoMedTech, Seoul, Korea) was used to measure the aggregation parameters of RBCs in vitro in whole blood samples [10]. Laser aggregometry is based on the diffused light scattering of a laser beam by the blood sample [11]. To perform the measurements 8 μL of whole blood were placed inside a flat reservoir and heated up to 37 ◦C. Then the sample was illuminated by a laser beam (633 nm, 2.5 mW), which was scattered by the RBCs and their aggregates mostly in the forward direction—the scattering particles were much larger than the light wavelength. The larger the size of the scattering particle the more intensity was scattered forward [12,13].

The time course of measured intensity of light scattered forward is presented in Figure 1. In the beginning of the measurement the RBCs were in a state of maximum aggregation and therefore the scattered intensity was also at its maximum. Then, a small magnetic bar inside the reservoir started stirring the sample, causing shear stress-induced destruction of the aggregates. After the stirring process (*t* = 0 in Figure 1), all aggregates were dispersed and none of the RBCs were in the aggregated state and therefore the scattered intensity was at its minimum; the cells themselves suffered no permanent damage from this. The stirring stopped and so the RBCs started to aggregate again, the average size of a scattering particle in the sample grew, and the scattered intensity increased. The aggregation process lasted approximately two minutes; after that the intensity reached its maximum, indicating that the cells were in a state of complete aggregation.

**Figure 1.** The kinetics of the RheoScan aggregometer output signal (intensity of light scattered forward as a function of time). The meaning of T1/2 and AI is indicated. 'A' is the area below the intensity curve inside the rectangle; 'B' is the area above the intensity curve inside the rectangle.

The aggregation kinetics were reflected in the dependence of the scattered intensity on time and several parameters were calculated based on it. Firstly, the characteristic time of aggregate formation (T1/2) characterized the time interval, during which the signal (scattered light intensity) reached half of the maximum value (see Figure 1). A smaller T1/2 indicated greater curve slope and faster aggregation of the cells. Secondly, the aggregation index (AI) characterized the fraction of cells aggregated during the first 10 s of measurement. It was calculated as a ratio between the area under the intensity curve to the total area above and below it (see Figure 1). Higher AI values corresponded to more numerous RBC aggregation in the sample.

#### *2.3. Laser Tweezers*

Laser tweezers (LT) are scientific tools that allow for the trapping and manipulation of microobjects (such as living cells, etc.) using a highly focused laser beam [14]. LT are essential instruments in single-cell studies. The physical principle of optical trapping is described in more detail in [15].

In our study, LT were used to measure the duration of the process of spontaneous aggregation of two individual RBCs [16]. Two beams from the Nd:YAG lasers (1064 nm, 200 mW) propagated through a system of lenses and polarizers and reached the dichroic mirror where they were split in two parts: The first one was directed to the aperture of the Olympus objective (×100, NA = 1.00, water immersion) and into the sample, and the second one to the photodetector in order to evaluate its power. One laser beam was always stationary whereas the other one could be moved by rotating the movable mirror—this allowed for two laser traps in the sample to be obtained: one stationary and one movable.

The measurements were carried out at room temperature (22 ◦C) in a highly diluted blood suspension inside a glass microcuvette with a 100 μm gap [17]. Patients' autological platelet-poor plasma was used as the suspension medium. The plasma was acquired by centrifuging all the blood for 10 min at 170 g, removing the platelet-rich plasma, then centrifuging the platelet-rich plasma for 10 min at 3000 g and removing the buffy coat. Lastly, the RBCs were added to the plasma to achieve the final hematocrit of about 0.1%. Due to such a high dilution of the suspension the hematocrit did not affect the measurements.

In LT the trapped RBCs oriented themselves vertically, so the cells were observed edge-on [18]. The time of doublet aggregate formation Tagg was measured by orienting two trapped RBCs parallel to each other and creating a single point of contact between their membranes using the movable laser trap (see Figure 2a) [16]. Then, the laser traps were disabled and the time of the doublet formation as a result of spontaneous aggregation was measured (see Figure 2b,c). Smaller values of Tagg corresponded to faster aggregate formation.

**Figure 2.** Three steps of Tagg measurement. Red crosses indicate the laser traps. (**a**) Two separate RBCs are brought together until the state of a "point contact"; (**b**,**<sup>c</sup>**) RBCs start to aggregate (overlap) after the laser beams are shut off.

For the interpretation of the results, it needs to be emphasized that the Tagg parameter corresponds to the initial stage of the aggregation process, whereas the laser aggregometry parameters (T1/2 and AI) represent the whole aggregation process, including the later formation of complex 3D aggregate structures.

#### *2.4. Digital Capillaroscopy*

Digital capillaroscopy was used to evaluate capillary blood flow parameters in vivo. Using the Kapillaroskan-1 device (AET, Moscow, Russia) a quantitative assessment of the blood flow characteristics was carried out in the nail bed capillaries. This method is described in more detail in [19,20]. Several nail bed capillaries of each patient were recorded at the high frame rate and then used to assess the average capillary blood flow velocity (CBV), which was calculated by frame-by-frame analysis.

Before the start of the measurements, the temperature of the skin of the studied finger was measured using an AND DT-635 skin thermometer (A&D, Tokyo, Japan). On average, the temperature of the skin of the finger in the patients included in the study was 33.6 ± 1.3 ◦C. There were no statistically significant differences between the groups considering the finger temperature.

#### *2.5. Statistical Analysis*

For each blood sample, the parameters AI T1/2, and Tagg were measured 5 times. The calculation of the CBV and the presence of aggregates for the DC method was carried out using original software that analyzed recordings of the nail bed capillaries. Videos of at least 6 good reading capillaries were used for calculations with a video duration of 3 to 5 s (at a recording rate of 100 frames per second, i.e., from 1800 to 3000 frames per patient). In the Results section the averaged values and the standard errors of the mean are presented. They were chosen over the standard deviations because they show the precision of the mean value. Statistical difference was calculated with a two-tailed Student *t*-test with unequal variance. The difference between the two values was considered statistically significant if the *p*-value according to the *t*-test was less than 0.05.
