Microcirculation plays a crucial role in tissue oxygenation and nutrient supply. Indeed, microvascular dysfunction may precede endothelial impairment in large arteries and clinical manifestations. It is becoming apparent that microcirculation is essentially involved in a variety of pathological conditions, and that microvascular dysfunction may be a biomarker in the development of cardiovascular disease [1]. Recently, accumulating evidence suggests that coronavirus disease 2019 (COVID-19) should be considered as a systemic microvascular endothelial disease with different clinical manifestations from severe and acute to completely asymptomatic course [2]. Hence, non--invasive and reliable methods for microcirculation status monitoring are still strongly needed.
Several methods are available to study the human microcirculation and to quantify microvascular blood flow. Among them, the recent non-invasive laser speckle contrast imaging (LSCI) provides a real-time monitoring of microvascular perfusion. Using LSCI, we showed that topical administration of treprostinil, a prostacyclin analog, increases cutaneous microvascular blood flow in diabetic patients [3]. Indeed, LSCI enables a precise quantification of variations of skin blood flow in two-dimension. LSCI measurements coupled with acetylcholine and sodium nitroprusside iontophoresis showed that for both agents the vasodilatation is reduced in early-onset coronary artery disease patients suggesting concurrent endothelial-dependent and -independent skin microvascular dysfunction [4]. Taken together, in clinical studies, LSCI is mainly used to assess skin microcirculation (Fig. 1) [5]. However, quite recently, LSCI was applied intraoperatively to estimate parathyroid viability [6]. Using two-dimensional LSCI, we recently performed non-invasive real-time microcirculation imaging on the beating heart (Fig. 2) in a patient undergoing coronary artery bypass grafting surgery [7].
Laser speckle contrast imaging is a recently developed technique based on speckle contrast analysis that provides an index of blood flow. When motionless tissue is illuminated with a laser, a random interference pattern, or speckle, is observed independent of the structure of the tissue surface. Speckle contrast is calculated as the ratio of its standard deviation to its mean intensity. When the laser light is scattered by moving red blood cells, the speckle pattern decorrelates. LSCI is based on the two-dimensional quantification of variations in this speckle contrast. Due to the movement of red blood cells, each single speckle intensity will fluctuate as a function of their velocity, and the time-integrated speckle contrast will be reduced. The penetration depth of LSCI measurements is about 300 μm, whereas it is deeper (about 1–1.5 mm) with laser Doppler techniques. Therefore, LSCI mostly records blood flow in the skin’s superficial papillary plexus while laser Doppler techniques record deeper dermal blood flow [8].
Laser speckle contrast imaging does not provide an exact measure of flow (mL/min). Measurements are therefore often expressed as arbitrary perfusion units or as cutaneous vascular conductance, which is flux divided by mean arterial pressure. The latter approach is more physiological as it takes into account differences and variations in blood pressure. Importantly, LSCI measurements can be carried out continuously, but are sensitive to movement artefacts.
In summary, LSCI allows non-invasive real-time monitoring of peripheral microcirculatory perfusion on a wide area of tissue with a very good spatial and temporal resolution and an excellent reproducibility. Therefore, LSCI combines the advantages of laser Doppler flowmetry and laser Doppler imaging [9]. As mentioned above, LSCI is mainly used in clinical studies to assess skin microcirculation [5]. However, LSCI is also successfully applied to animal studies and angiogenesis measurements [10].
A number of common clinical conditions are closely associated with microvascular dysfunction. The monitoring of the microvascular perfusion is therefore of essential interest in various experimental and clinical studies. LSCI measurements are reproducible and highly sensitive to acute changes in tissue perfusion. Of note, this technique coupled with vascular reactivity tests enables assessment of endothelial function. Additionally, LSCI can be easily applied in pharmacological studies aimed at assessing drug safety, efficacy and influence on microcirculation in cardiovascular diseases [3].