Experimental acute myocardial infarction
Experimental acute myocardial infarction:telocytes involvement in neo-angiogenesis
C. G. Manole a, b , V. Cisma?s iu b , Mihaela Gherghiceanu b , L. M. Popescu a, b, c, *
a
Department of Cellular and Molecular Medicine, ‘Carol Davila’ University of Medicine and Pharmacy, Bucharest, Romania b
Division of Advanced Studies, ‘Victor Babe?s ’ National Institute of Pathology, Bucharest, Romania
c
National Academy of Sciences, Bucharest, Romania
Received: April 20, 2011; Accepted: August 25, 2011
Abstract
We used rat experimental myocardial infarction to study the ultrastructural recovery, especially neo-angiogenesis in the infarction border zone. We were interested in the possible role(s) of telocytes (TCs), a novel type of interstitial cell very recently discovered in myocardim (see https://www.wendangku.net/doc/453855004.html,). Electron microscopy, immunocytochemistry and analysis of several proangiogenic microRNAs provided evi-dence for TC involvement in neo-angiogenesis after myocardial infarction. Electron microscopy showed the close spatial association of TCs with neoangiogenetic elements. Higher resolution images provided the following information: (a) the intercellular space between the abluminal face of endothelium and its surrounding TCs is frequently less than 50 nm; (b) TCs establish multiple direct nanocontacts with endothelial cells, where the extracellular space seems obliterated; such nanocontacts have a length of 0.4–1.5 ?m; (c) the absence of basal membrane on the abluminal face of endothelial cell. Besides the physical contacts (either nanoscopic or microscopic) TCs presum-ably contribute to neo-angiognesis via paracrine secretion (as shown by immunocytochemistry for VEGF or NOS2). Last but not least,TCs contain measurable quantities of angiogenic microRNAs (e.g.let-7e, 10a, 21, 27b, 100, 126-3p, 130a, 143, 155, 503). Taken together,the direct (physical) contact of TCs with endothelial tubes, as well as the indirect (chemical) positive influence within the ‘angiogenic zones’, suggests an important participation of TCs in neo-angiogenesis during the late stage of myocardial infarction.
Keywords: acute myocardial infarction ?neo-angiogenesis ?telocytes ?endothelial cells ?microRNAs ?angiogenic zones ?
VEGF ?NO synthase 2 ?cardiomyocytes
J. Cell. Mol. Med. Vol 15, No 11, 2011 pp. 2284-2296
? 2011 The Authors
Journal of Cellular and Molecular Medicine ? 2011 Foundation for Cellular and Molecular Medicine/Blackwell Publishing Ltd
doi:10.1111/j.1582-4934.2011.01449.x
Introduction
Understanding the mechanisms of cardiac regeneration and repair after myocardial infarction is an important subject of contempo-rary medicine. The effects of experimental myocardial infarction were frequently reported [1–16]. Indeed, according to PubMed database, there are 3840 titles (from 1956 to August 2011) for the ‘rat myocardium infarction’ search! E xperimental myocardial infarction shows two different zones: (a) the central zone where most of the normal myocardial components (cardiomyocytes –CMs, interstitial cells, capillaries) are disintegrated; (b) the border zone with acute hypertrophy, followed by chronic hypertrophy (even after the healing process is over), and tissue remodelling.
Previously, our group documented the presence of a distinct interstitial cell type in heart [17–19]. The term telocyte (TC) was coined for these cells, and telopodes (Tps) for their very long (tens to hundreds of ?m) and moniliform prolongations [20–23]. Tps are an alternation of thin segments (podomers) and dilated seg-ments (podoms). Podomers are very thin (up to 0.2 ?m), below the resolving power of light microscopy, explaining the fact that TCs were overlooked [20–23]. The concept of TC was taken up by other Laboratories [24–36]. Moreover, Liu et al.[37] reported the distribution of TCs in rat heart: more in atria than in ventricles (20versus 9 cells/mm 2) and significantly higher in subepicardium than in endocardium (18 versus 7 cells/mm 2).
The aim of this study was to assess the involvement of TCs in the neo-vascularization process in the border zone of infarction. By electron microscopy and immunocytochemistry we observed TCs in the border zone 30 days after myocardial infarction. TCs appear in close spatial relationships with blood vessels and immunopositive
JCMM Express *Correspondence to: L.M. POPESCU, M.D., Ph.D., Department of Cellular and Molecular Medicine, “Carol Davila” University of Medicine and Pharmacy, P .O. Box 35-29, Bucharest 35, Romania. E-mail: LMP@https://www.wendangku.net/doc/453855004.html,
J. Cell. Mol. Med. Vol 15, No 11, 2011
2285
? 2011 The Authors
Journal of Cellular and Molecular Medicine ? 2011 Foundation for Cellular and Molecular Medicine/Blackwell Publishing Ltd
for VEGF and NOS2. By microRNA qPCR we found, at the level of TC body, the expression of various angiogenic microRNAs.Therefore, TCs appear as key-players in neo-angiogenesis within the ‘angiogenic zones’ of the border zone infarction.
Materials and methods
Rat surgery
A number of four Wistar male rats (average weight of 270 g) have under-gone surgery for ligation of left anterior descending coronary artery (LADC), in accordance with the Institutional Ethical Committee approval.For rat myocardial infarction the experimental protocol was adapted from that used by Od?rfer et al.[38].
One day before surgery, each animal received injectable antibiotic enrofloxacin (Baytril; Bayer, Leverkusen, Germany) and pretreated metami-zol sodium (Algocalmin; Zentiva, Bucharest, Romania). Anaesthesia was made with a cocktail consisting of acepromazine maleate (Neurotranq;Alfasan, Woerden, Holland) and Ketamine hydrochloride (Ketamine HCL ?;Kepro, Deventer, Holland). Animals were intubated using a Teflon catheter (16G/?1.7; Suru International Pvt. Ltd., Mumbai, India). Each animal was positioned on the right side on a 38?C heat-held plate (Harvard Apparatus,Holliston, MA, USA). During the surgery each animal was connected to a ventilator CWE SAR-830/P ventilator (Ardmore, PA, USA) with external air pump (ASF Inc, Norcross, GA, USA), set at a rate of 52 breaths per minute with a volume of 8 ml of air. After the surgical tolerance was examined and no more control reflexes were triggered, the thorax was opened between the third and fourth ribs, by blunt splitting of the Mm. intercostales.Pericardium was opened and arteria coronaria sinistra was proximally sur-rounded Vicryl 5-0 (SMI, Hünningen, Belgium) with a surgical knot. In all cases the ligation was made immediately below the lower margin of the left auricle. The acute occlusion of LADC of the ligature was verified by the pal-lor of the unsupplied myocardium. The closure of the chest was performed using 3–4 stitches Vicryl 4-0 (SMI, Hünningen, Belgium) between cranial and caudal ribs. The lung was previously expanded to prevent pneumoth-orax. Each muscular layer was continuously sutured with Vicryl 4-0 (SMI,Hünningen, Belgium). The surgical wound was bacteriostatic covered with oxytetracycline (Oxyvet, Veterin, Attiki, Greece). After the surgery, the ani-mal was disconnected from the ventilator and extubated. Once the reflexes appeared, the animal was moved in a cage with sterile wood chips.Subsequently, the animal received metamizole sodium (Algocalmin;Zentiva, Bucharest, Romania) for immediate analgesia. The aftercare med-ication was for 3 days after the surgery, contained enrofloxacin, for antibi-otic therapy and sodium metamizole for pain therapy.
The LV dysfunction in this experimental model of rat myocardial infarction was assessed by echocardiography, using a Vevo 770 Imaging System (Visualsonics, Toronto, Canada) with a 15–22.5 KHz transducer.
Transmission electron microscopy
Thirty days after permanent ligation of the LADC, the rats were killed by cervical dislocation. The hearts were harvested. Small fragments (1 mm 3)of rat ventricular myocardium (infarction area and border zone) were processed for transmission electron microscopy (TEM) according to rou-tine E pon-embedding procedure, previously described [17, 19, 39–41].
The thin and thick sections were cut with a diamond knife using an RMC ultramicrotome (Boeckeler Instruments, Inc., Tucson, AZ, USA) and dou-ble-stained with 1% uranyl acetate and Reynolds lead citrate. Sections of about 60-nm-thin were examined with a Morgagni 286 transmission elec-tron microscope (FE I Company, E indhoven, The Netherlands) at 60 kV.Digital electron micrographs were recorded with a MegaView III CCD using iTE M-SIS software (Olympus, Soft Imaging System GmbH, Monster,Germany). On TEM images TCs, Tps, blood vessels were digitally coloured in blue and brown using Adobe ?Photoshop CS3 to mark them out.
Immunocytochemistry
Immunohistochemistry for VE GF and NOS2 was done according to the protocol reported by Suciu et al.[42] and Popescu et al.[43].
Laser capture microdissection (LCM), RNA isolation and microRNA qPCR
Cell cultures and methods used were previously described [44]. Cells were fixed with absolute ethanol and stained with Giemsa. LCM was performed using the PALM MicroBeam system (Carl Zeiss MicroImaging GmbH, Jena,Germany) in accordance with the manufacturer protocols. For each sam-ple, TC and control, a total of 500 cells were harvested in two separate experiments. The catapulted cells were captured and lysed in E pp tube caps filled with 30 ml of TRI Reagent (Sigma-Aldrich, St. Louis, MO, USA).Total RNA was extracted using the standard protocol recommended by the manufacturer (Sigma-Aldrich). The purity of RNA was evaluated with the NanoDrop ND-1000 Spectrophotometer (Thermo Scientific, Waltham, MA,USA). For cDNA synthesis we used QuantiMir RT (System Biosciences,San Francisco, CA, USA) according to manufacturer instructions. The cDNA templates were then quantified in a real-time SYBR Green qPCR reaction (iCycler system and software, Bio-Rad, Hercules, CA, USA) using universal reverse primers and microRNA-specific forward primers (System Biosciences, San Francisco, CA, USA). Mouse U6 snRNA and RNU43 were used as endogenous controls. The negative control was performed by omitting the reverse transcriptase.
Statistics
The data are represented as mean ?S.D. of three experiments and two-tailed P values of less than 0.05 were considered as statistically significant.
Results
In all the cases the central zone and the corresponding border zone of infarction were clearly distinguishable. The lesion develop-ment corresponded to that previously described in literature.Figures 1–4 show TEM modifications of the border zone at specific intervals after LADC ligation: 1 day, 2 days, 1 week and 1 month.Figure 1 shows an area of border zone of myocardial infarction,1 day after the ligation of LADC. The general aspect is typical for an acute inflammatory reaction . The dominant population is
2286
? 2011 The Authors
Journal of Cellular and Molecular Medicine ? 2011 Foundation for Cellular and Molecular Medicine/Blackwell Publishing Ltd
represented by granulocytes: eosinophils and polymorphonuclear neutrophils. The lumen of capillaries is dilated, presumably due to the hypoxic conditions at the level of the border zone. Apparently,TCs are not so frequently found like in normal myocardium.However, we did not make a quantitative comparison.
Figure 2 shows a TE M aspect from the border zone, 2 days after the ligation of LADC. The most visible modification is fibrob-last proliferation . Incidentally, Figure 2 presents three typical fibroblasts and three CMs. However, in normal myocardium the ratio fibroblasts:CMs is not 1:1 (!). Noteworthy, a previous study of our Laboratory [45] reported a morphometric results, by stere-ology, which indicated that CMs in rat ventricular myocardium occupy 76% and fibroblasts only 1.5% of myocardial volume (the remaining percentage corresponds to extracellular matrix,endothelial cells, TC and other interstitial cells). Thus, in our opin-ion, after 2 days of myocardial infarction the dominant phenome-non is the beginning of fibrosis , which is primarily produced by fibroblast proliferation. Again, TCs presence seems to be not so frequent like in normal myocardium, but no direct quantitative comparison was made.
Figure 3 demonstrates the presence of myofibroblasts (cells
which share features with Fb and with smooth muscle cells [46])
Fig. 1 Rat experimental myocardial infarc-tion. Border zone: 1-day-old. Transmission electron microscopy. The inflammatory granulocyte reaction dominates: granulo-cyte infiltration, mainly eosinophils (E) and neutrophils (PMN); a mast cell (M) is visi-ble; the arrow indicates an apoptotic cell. A telocyte (TC) and several telopodes (Tp) are
digitally blue coloured.
Fig. 2 Rat experimental myocardial infarc-tion. Border zone: 2-day-old. Transmission electron microscopy. Three fibroblasts (upper part) intermingle with three car-diomyocytes (lower part). The accumula-tion of fibroblasts indicates the beginning of fibrosis. Note that usually, in normal myocardium, there are no fibroblast clus-ters; Fb: fibroblast; rER: rough endoplasmic reticulum; Eu-N: euchromatin; n: nucleolus;CM: cardiomyocyte; m: mitochondria; Z: Z line. Centriole presence (black dotted line)suggests fibroblast mitosis. Tp: telopode (digitally blue coloured); E: eosinophil.
J. Cell. Mol. Med. Vol 15, No 11, 2011
2287
? 2011 The Authors
Journal of Cellular and Molecular Medicine ? 2011 Foundation for Cellular and Molecular Medicine/Blackwell Publishing Ltd
in the border zone, seven days after the acute occlusion of LADC.Abundant rE R is obvious (like in active fibroblasts), as well as myofilaments and caveolae (like in smooth muscle cells).Moreover, this myofibroblast presents a very characteristic fea-ture: a cell-to-matrix adhesive structure – fibronexus (Fig. 3) –which enables the positive diagnostic [47, 48]. The myofibroblasts are particularly responsible for matrix remodelling .Thirty days after the LADC ligation, a process of recovering char-acterizes the border zone of the myocardial infarction (Fig. 4). CMs begin to have normal ultrastructural appearance. In the interstitium,the number of TCs is clearly increased in comparison with normal myocardium. TCs/Tps have close spatial relationships with blood capillaries. However, the distances separating the Tps and abluminal
front of endothelial cells and Tps are different for capillary of neo-Fig. 3 Rat experimental myocardial infarc-tion. Border zone: 7-day-old. Transmission electron microscopy. Note the presence of a typical myofibroblast. Such cells are responsible for matrix remodelling.Myofibroblasts have intermediate features between fibroblasts and smooth muscle cells: prominent rough endoplasmic reticu-lum (rE R, like fibroblasts), and myofila-ments (mf, like smooth muscle cells)located under the cell membrane. The char-acteristic ultrastructural feature, the fibronexus, which is a cell-to-stroma attachment, is highlighted by black dotted
circle. E: eosinophil; coll: collagen fibrils.
Fig. 4 Rat experimental myocardial infarction. Border zone: 30-day-old.Transmission electron microscopy. This low magnification view shows four car-diomyocytes (CM), two blood capillaries (1 and 2) and numerous telocytes (TC) with long and slender telopodes (Tp). Note the close spatial relationship between TC/Tp and capillary-1 wall (endothelium).Capillary-1 is presumably a neo-capillary created in the interstitial space. Capillary-2,between three cardiomyocytes (CMs), has a TC and Tps in the vicinity, but the distance between abluminal membrane of endothe-lium and TC/Tp plasma membrane is wider.Thus, capillary-2 is probably an ‘old’capillary.
2288
? 2011 The Authors
Journal of Cellular and Molecular Medicine ? 2011 Foundation for Cellular and Molecular Medicine/Blackwell Publishing Ltd
formation (e.g.capillary-1 in Fig. 4) versus preexisting capillaries (e.g.capillary-2 in Fig. 4). Digitally measurements of the nanoscopic and microscopic distances resulted in the following results:
(a)Capillary of neo-formation:there are two situations:
i.ither the extracellular space between abluminal endothelial cell membrane and the Tp membrane is oblit-erated, both membranes coming in direct physical con-tact (less than 10 nm);
ii.A very narrow intercellular cleft (comparable with canon-ical synaptic cleft !) with dimensions ranging between:- a minimum of about 80 nm (red dots in Fig. 4), and - a maximum of about 120 nm (orange dots in Fig. 4).(b) Preexisting capillaries:the widths of spaces separating the two plasma membranes (endothelial and telopodic) are wider, being around 200 nm (below the practical resolving power of light microscopy).
Figure 5 shows ultrastructural modifications in the central zone , after 30 days of myocardial infarction (compare with the ‘border zone’ of Figs 1–4). Abundant deposits of collagen are visible. CMs have discontinuous Z lines and myofibrils look ‘homogenized’. Cells have some characteristics of apoptosis :shrinkage of the cells, condensation of chromatin, cellular frag-mentation (observable at cellular poles, mainly). Apoptotic bodies can also be seen. The dyskinetic areas of infarction (like in Fig. 5)were documented by echocardiography and ECG. Figure 6 corre-sponds to the functional damage of the left ventriculum, as a result of LADC ligation.
Figures 7 and 8 provide additional evidence for the involvement of TCs in neo-angiogenesis after 30 days of myocardial infarction.The number of TCs and Tps is increased in the border zone. Their close spatial relationships with new-formed blood capillaries is obvious. In Figure 7, Tp1 surrounds and establishes multiple nanocontacts with the new-formed capillary. The length of these contacts ranges between 0.36 and 1.45 ?m, as it is shown at
higher magnification in Figure 8. The width of the space between
Fig. 5 Rat experimental myocardial infarc-tion. Central zone of the scar: 30-day-old;transmission electron microscopy. Three structural elements can be recognized in this image: (a) abundant deposits of collagen fib-rils (coll), cross or obliquely cut; (b) dam-aged cardiomyocytes (CM), ‘homogenized’myofibrils, only positions of Z lines being recognizable; (c) apoptotic interstitial cells
(IC), and apoptotic bodies.
Fig. 6 Typical echocardiogram of rat experimental myocardial infarction (30-day-old). The black arrow indicates the dyskinetic region of ventricular free wall corresponding to myocardial infarction area. The corresponding ECG in the lower part of the figure shows typical elevation of ST segment,suggestive for acute myocardial infarction.
J. Cell. Mol. Med. Vol 15, No 11, 2011
2289
? 2011 The Authors
Journal of Cellular and Molecular Medicine ? 2011 Foundation for Cellular and Molecular Medicine/Blackwell Publishing Ltd
Fig. 7 Rat experimental myocardial infarction. Border zone: 30-day-old. Transmission electron microscopy. A new-formed blood capillary with an anfrac-tuous and narrow lumen is shown (brown colour) in the mass of collagen fibrils (coll) of the scar. This is surrounded by two telocytes (TC1 and TC2 -blue colour) and their corresponding telopodes (TP1 and Tp2). Typically podoms (dilated portions) and the intercalary podomers (thin portions of Tp)can be observed. At the level of podoms there are many mitochondria (m), elements of endoplasmic reticulum and caveolae. Note the close spatial rela-tionships between telopodes and endothelial cells. The space between telopodes and the membrane of endothelial cell is occasionally less than 50 nm
and there is no visible endothelial basal lamina.
Fig. 8 Higher magnification of the fields marked by colour rectan-gles in Figure 7. (A ) A nanocontact of about 1.45 μm long between the telocyte (TC) and the membrane of the endothelial cell (E ) is marked by the green dotted line. The asterisk indicates the intercel-lular space between TC and E. No endothelial basal lamina is pres-ent. (B ) A nanocontact of about 0.45 mm long between the E and TC is indicated by the red dotted line. The asterisk mark intercellu-lar space without endothelial basal membrane and the two arrows show possible electron dense ‘feet’ connecting the endothelial cell membrane and the TC membrane. (C ) A nanocontact of 0.36 mm long between endothelial cell membrane and TC is indicated by yel-low dotted line between the endothelial cell membrane and TC membrane. No basal lamina is visible in the extracellular space between the endothelium and TC (asterisks).
2290
? 2011 The Authors
Journal of Cellular and Molecular Medicine ? 2011 Foundation for Cellular and Molecular Medicine/Blackwell Publishing Ltd
Fig. 9 Rat experimental myocardial infarction. Border zone: 30-day-old. Transmission electron microscopy. Telopodes (Tp) are situated in close vicinity of blood vessels. Vascular smooth muscle cells (VSMC) and endothelial cells (End) have many caveolae. Note the alternation of podoms and podomers. Podoms contain: mitochon-dria (m), and endoplasmic reticulum (ER) and caveolae (cav). (A )Shed vesicles (sv) are released from podoms. A vesicle cargo mul-tivesicular is formed from a podomer (B ) and another one is formed from a podom (C ). coll: collagen.
the plasma membrane of the Tp and the endothelial cell membrane is 50–70 nm (Fig. 8B) or 40–100 nm (Fig. 8C). Within the extra-cellular space some electron-dense ‘feet’, with a ‘height’ of about 60 nm, seem connect endothelial and TC cell membranes. The endothelial basal lamina is absent along these nanocontacts .In the vicinity of new-formed blood capillaries, TCs and Tps release shed vesicles and vesicle groups from podoms and/or podomers (Fig. 9). In Figure 9A, the visible shed vesicles have a diameter between 60 and 330 nm. The vesicle groups in Figure 9B and C are of 730/280 nm and 710/470 nm, respectively. They have a heterogeneous content and seem to be involved in heterocellu-lar communication.
For underlining the involvement of TC in angiogenesis, Figures 9 and 10 show the strategic positions of the Tps either among new-formed blood vessels (Fig. 9), or surrounding them (Fig. 10).The new-formed blood vessels have typical tall endothelial cells with numerous organelles and a narrow and anfractuous lumen (Figs 11 and 12). The endothelium has many transcytosis vesicles.
Immunocytochemistry performed show positive reactions of TC for VE GF and NOS2 in normal heart (Fig. 13). In the border zone of the myocardial infarction positive expression for both VEGF and NOS2 is shown by cells with similar appearance with
Fig. 10 Rat experimental myocardial infarction. Border zone: 30-day-old. Transmission elec-tron microscopy. A telopode (Tp - blue colour) is located between three new-formed capillar-ies (cap). At the level of capillary A, basal lamina and fragments of pericytes (asterisks) are visible. The capillary endothelium (brown colour) has many vesicles of transcytosis. Note the alternation of podoms (containing mitochondria, endoplasmic reticulum and caveolae) and podomers (thin segments) – arrows.
J. Cell. Mol. Med. Vol 15, No 11, 2011
2291
? 2011 The Authors
Journal of Cellular and Molecular Medicine ? 2011 Foundation for Cellular and Molecular Medicine/Blackwell Publishing Ltd
TC. These cells are located in the close vicinity of blood vessels having close spatial relationships with them.
Because the data suggest that TCs are intimately connected with the neovascularization after myocardial infarction, we have investigated whether TCs are expressing angiogenic microRNAs.Cardiac TCs were isolated from the first-passage cultures by laser capture microdissection (Fig. 14) and the expressions of microRNAs were determined by RT-qPCR as previously described [41]. The data presented in Figure 15 show that several microRNAs with angiogenic functions are present in TCs.
Discussion
Angiogenesis is essential for myocardium repair and remodelling after myocardium infarction. Direct intercellular communication of endothelial cells with other cells is crucial for an efficient vascular formation [49]. The direct contact of endothelial progenitors with
‘ventricle slices’ (presumably TC !?) seems of importance for angiogenesis [50].
It is widely accepted that after 30 days of experimental myocar-dial infarction, the border zone of the lesion is characterized by neo-angiogenesis [13, 51]. Generally, there are many types of angiogenic factors: e.g.(a) growth factors and their receptors; (b)matrix proteins and proteases; (c) adhesion molecules; (d)microRNAs and transcription factors.
We used a trio of methods (morphology – transmission elec-tron microscopy; immunocytochemistry – VE GF and NOS2expression and molecular biology – angiogenic microRNAs expression), which showed the involvement of TC in neo-angio-genesis, in the border zone.
Electron microscopy
In the border zone of myocardial infarction the relationships between TCs and new-formed blood vessels are obvious. TCs have close vicinity with new-formed blood vessels (capillary and/or arterioles), but also with the preexisting blood vessels.The space between TCs/Tps and the abluminal face of the endothelium is sometimes less than 50 nm, and therefore in the macromolecular-interaction range. Anyway, TCs establish heterocellular contacts also with CM as it was previously described [52].
TCs/Tps release shed vesicles or exosomes. The roles of exosomes are not understood, but they seem to play an impor-
tant role in intercellular communication [53]. Shed vesicles
Fig. 11 Rat experimental myocardial infarction. Border zone: 30-day-old.Arteriologenesis. Transmission electron microscopy. A telopode (Tp) sur-rounding a new-formed blood vessel. Tall endothelial cells (End) with numer-ous mitochondria (m) and endoplasmic reticulum (ER) cisternae, circumvent
a narrow and irregular lumen (L). VSMC: vascular smooth muscle cell.
Fig. 12 Rat experimental myocardial infarction. Border zone: 30-day-old.Arteriologenesis. Transmission electron microscopy. Telopodes (Tp) with typical podoms and podomers, from at least one telocyte (TC - blue colour)are encircling an arteriole (A: brown colour). Note: (a) the endothelium (brown coloured) surrounding the lumen which contains a red blood cell (RBC: red colour); (b) lamina elastica interna – a clear space surrounding the endothelium; (c) 2–3 layers of smooth muscle cells (SMC).
2292
? 2011 The Authors
Journal of Cellular and Molecular Medicine ? 2011 Foundation for Cellular and Molecular Medicine/Blackwell Publishing Ltd
and exosomes presumably transfer macromolecules (e.g.microRNAs, proteins), which cannot be released through the intact plasmalema. Our results suggest some possible mecha-nisms for TCs involvement in ‘angiogenic zones’: either direct (physical contact), or indirect (chemical signalling) (Fig. 16). An ‘exosome therapy’ could be taken into account as a future pos-sibility [54, 55].
Immunocytochemistry
Immunocytochemistry done for NO and VEGF confirmed our pre-vious studies regarding the presence of TC in normal myocardium.After 30 days of myocardial infarction, interstitial cells similar to those described in normal heart are found in affected myocardium.At the level of cell body and cell prolongations these cells have pos-itive expression for NO and VEGF, as it was previously reported in other organs [41–43]. These data could be relevant because TC may promote and/or modulate angiogenesis after myocardial infarction via VEGF and/or NO secretion.
Angiogenic microRNAs
The human genome encodes 1048 microRNAs, which virtually reg-ulate all biological processes [56]. In addition, microRNAs are pre-dicted to regulate the expression of more than one-third of human protein-coding genes. There is increasing evidence that miRNAs
play important roles in vascular development as well as in vascular diseases. Here we show that several pro-angiogenic microRNAs are expressed by TCs: e.g.miR 126 [57], miR130a [58], let-7 fam-ily [59, 60], miR-10 [61], miR-155 [62], miR-503 [63]. Another pro-angiogenic factor, miR-21, induces HIF-1?and VEGF expres-sion and activates both AKT and E RK pathways for mediating angiogenesis [64]. The clusters of miRNAs which include miR-27are highly expressed in ECs and repress the anti-angiogenic pro-teins Sprouty2 and Sema6A [65]. The proliferation, migration and tube formation of ECs are regulated also by miR-100 [66]. Also,miR-143 is abundant microRNA in vascular smooth muscle cells and it was found down-regulated in diseased arteries [67].
Interestingly, TCs express both stromal specific [44] and vas-cular smooth muscle specific (miR-143/145) microRNAs as well as pro-angiogenic miRs highly enriched in endothelial cells (such as miR-126). Such expression patterns may support the view that several cell type specific signalling pathways converge in TCs and further suggests a complex regulatory mechanism driven by telocytes during the cardiac regeneration. In addition, TCs may secrete microvesicles or exosomes containing specific cocktail(s)of miRNAs, which are internalized by surrounding cells (such and endothelial and smooth muscle cells). Thus, these cells can mod-ulate the angiogenesis process through paracrine signals.
Figure 16 presents the essential data of our results and propos-als for the mechanisms involved in neo-angiogenesis in the border zone of myocardial infarction, including the microRNA participation via secretion (transport by shed vesicles and/or
exosomes), that we call ‘microcrine’ phenomenon. The possible
Fig. 13 Rat normal heart tissue (A , B ) and border zone of infarcted heart tissue (C , D ) in experimental myocardial infarction (30-day-old). (A ) Immunostaining for VEGF demonstrates positive expression in the subepicardial area. A silhouette of a telocyte (TC) can be seen parallel with the epicardium. Very long and slender telopodes (Tp) are obvious. (B ) Positive expression for NOS2 in rat normal myocardium. A Tp splits dichotomously near the TC cell body, and runs parallel with cardiac fibres. (C ) In the border zone of infarcted heart tissue, near a new-formed arteriole (A ), a cell (most probable a TC,taking into account the morphology) is positive for VE GF (arrow). (D ) Positive reaction for NOS2 in two different cells (arrows) near a new-formed blood vessel in the border zone of infarction. Their prolon-gations are neighbouring the blood vessel wall. Original magnifications: (A , B ) – 100?;(C , D ) – 60?.
J. Cell. Mol. Med. Vol 15, No 11, 2011
2293
? 2011 The Authors
Journal of Cellular and Molecular Medicine ? 2011 Foundation for Cellular and Molecular Medicine/Blackwell Publishing Ltd
role(s) of TC in the maturation of capillaries into arteriolar vessels remains to be established.
There is a good correlation between electron microscopy and immunocytochemistry because it is well known that experimen-tally induced ischaemia results in a dramatic increase of VEGF lev-els in myocardium [68, 69]. Moreover, VE GF appears to act by local up-regulation of NO production [70, 71].
Since telocytes are CD34 positive [20, 23, 41, 43], our results support the assumption of Kumar & Caplice [72] that paracrine factors secreted by CD34 positive cells contribute significantly to angiogenesis. Moreover, very recently Sahoo et al.[73]demonstrated that CD34 positive cells secrete vesicles (exosomes)that have independent angiogenic activity, both in vitro and in vivo .But Figure 9 (A-C) shows directly by electron microscopy that TCs release shed vesicles and group of such vesicles (as multivesicular bodies) in angiogenic areas of the myocardial infarction border zone. This may not be a simple coincidence.
Further studies are required to clarify the relationships between TCs and pericytes, because pericytes are cells involved in angiogen-esis, too [74, 75]. Anyway, preliminary studies in our Laboratory showed that TC are PDGF-R positive, like pericytes, in other words PDGF-R is not a marker for pericytes (Popescu et al.
, in preparation).
Fig. 15 Expression levels of microRNAs up-regulated in telocytes. The relative expression was determined by real-time PCR. RNU43 snoRNA and U6 snRNA were used as normalizing controls. The error bars are mean ?S.D. (n ?3) and the data are representative
for two replicate experiments. AU: arbitrary units.
Fig. 14 Laser capture microdissection of cardiac telocytes in culture. Because other interstitial cells than telocytes might be present, only cells with ‘multi-polar’ body and at least one prolongation of more than 50 mm long were considered telocytes. Such prolongations had typical telopode conformation, with podoms (dilated portions) and podomers (thin segments). (A ) The telocyte body encircled by the red line was dissected out by laser capture microscopy.(B ) The corresponding area of Figure 11A after microdissection. A total of 500 telocyte bodies were collected and analysed for microRNAs. 20?objective.
2294
? 2011 The Authors
Journal of Cellular and Molecular Medicine ? 2011 Foundation for Cellular and Molecular Medicine/Blackwell Publishing Ltd
Finally, we support the idea of Laflamme and Murry [36] that ‘after more than a decade of furious activity’ stem cells … and neo-angiogenesis … ‘seem to be catching up with its promise’. A TC-based therapeutic neo-angiogenesis in myocardial infarction could have a significant clinical potential.
Acknowledgements
The authors thank Professor árpád Tósaki and Dr. Juhász Béla (Department of Pharmacology and Pharmacodynamics, University of
Debrecen, Hungary) for their constant help in realizing the echocardiogra-phy for operated rats. This paper is partially supported by the Sectorial Operational Programme Human Resources Development (SOPHRD),financed from the E uropean Social Fund and by the Romanian Government under the contract number POSDRU/89/1.5/S/64153(V.B.C.). Prof. L.M. Popescu thanks Cord Blood Center (Cluj) for financial assistance.
Conflict of interest
The authors declare no conflicts of interest.
References
1.
Caulfield J, Klionsky B.Myocardial ischemia and early infarction: an electron
microscopic study . Am J Pathol.1959; 35:
489–523.
2.
Page E, Polimeni PI.Ultrastructural
changes in the ischemic zone bordering
experimental infarcts in rat left ventricles .Am J Pathol.1977; 87: 81–104.
3.
Gottlieb GJ, Kubo SH, Alonso DR.Ultrastructural characterization of the border zone surrounding early experimental myocardial infarcts in dogs. Am J Pathol . 1981; 103:
292–303.
4.
Axford-Gatley RA, Wilson GJ.The “bor-der zone” in myocardial infarction. An ultrastructural study in the dog using an
electron-dense blood flow marker. Am J Pathol . 1988; 131: 452–64.
5.Schaper J.Ultrastructural changes of the myocardium in regional ischaemia and infarction. Eur Heart J.1986; 7B: 3–9.
6.Vracko R, Thorning D.Contractile cells in rat myocardial scar tissue. Lab Invest.1991; 65: 214–2
7.
7.Matsushita T, Oyamada M, Fujimoto K,et al .Remodeling of cell-cell and cell-extracellular matrix interactions at the bor-der zone of rat myocardial infarcts. Circ Res.1999; 85: 1046–55.
8.Frangogiannis N G, Smith CW, Entman ML.The inflammatory response in myocar-dial infarction. Cardiovasc Res.2002; 53:31–47.
9.
Wang B, Ansari R, Sun Y, et al .The scar neovasculature after myocardial infarction in rats. Am J Physiol Heart Circ Physiol.2005; 289: H108–13.
10.Weber KT, Sun Y, Dìez J.Fibrosis: a living
tissue and the infarcted heart . J Am Coll Cardiol.2008; 52: 2029–31.
11.Zornoff LA, Paiva SA, Minicucci
MF, et al .xperimental myocardium infarction in rats: analysis of the model.Arq Bras Cardiol.2009; 93: 434–40, 426–32.
12.Bharti S, Arora S, Arya DS.Evaluation of
morphological changes in experimental models of myocardial infarction: electron and light microscopical evidence. In: A. Méndez-Vilas, J Díaz, editors.Fig. 16
Possible mechanisms of telocyte involvement in neo-angiogenesis in the border zone of myocardial infarction.
J. Cell. Mol. Med. Vol 15, No 11, 2011
2295
? 2011 The Authors
Journal of Cellular and Molecular Medicine ? 2011 Foundation for Cellular and Molecular Medicine/Blackwell Publishing Ltd
Microscopy: science, technology, applica-tions and education. Formatex, Spain;2010. p. 361–71.
13.Jin P , Wang E, Wang YH, et al .Central zone of myocardial infarction: a neglected target area for heart cell therapy. J Cell Mol Med.2011; doi: 10.1111/j.1582–4934.2011.01408.x.
14.Ye KY, Black LD 3rd.Strategies for tissue engineering cardiac constructs to affect functional repair following myocardial infarction. J Cardiovasc Transl Res.2011;doi: 10.1007/s12265-011-9303-1.
15.
Wang H, Liu Z, Li D, et al .Injectable biodegradable hydrogels for embryonic stem cell transplantation: improved car-diac remodeling and function of myocar-dial infarction. J Cell Mol Med . 2011; doi:10.1111/j.1582-4934.2011.01409.x
16.
Wu Y, Yin X, Wijaya C, et al .Acute myocardial infarction in rats. J Vis E xp.2011; 48: 2464; doi: 10.3791/2464.
17.Popescu LM, Manole CG, Gherghiceanu M, et al .Telocytes in human epicardium.J Cell Mol Med.2010; 14: 2085–93.
18.
Gherghiceanu M, Popescu LM.Cardiomyocyte precursors and telocytes in epicardial stem cell niche: electron micro-scope images. J Cell Mol Med.2010; 14:871–7.
19.
Gherghiceanu M, Manole CG, Popescu LM.Telocytes in endocardium: electron microscope evidence. J Cell Mol Med.2010; 14: 2330–4.
20.
Popescu LM, Faussone-Pellegrini MS.Telocytes – a case of serendipity: the wind-ing way from interstitial cells of Cajal (ICC), via interstitial Cajal-like cells (ICLC)to telocytes . J Cell Mol Med.2010; 14:729–40.
21.
Popescu LM.Telocytes – a novel type of interstitial cells. In: Braisant O, Wakamatsu H, Kang I, Allegaert K, Lenbury Y, Wacholtz A, editors. Recent researches in modern medicine -HISTEM’11. Cambridge: WSEAS Press; 2011. p. 424–32.
22.Popescu LM.The tandem: telocytes –stem cells. Intl J Biol Biomed Eng.2011; 2:83–92.
23.
Faussone-Pellegrini MS, Popescu LM.Telocytes. BioMol Concepts.2011; doi:10.1515/BMC.2011.039.
24.
Gittenberger-de Groot AC, Winter EM,Poelmann RE.E picardium-derived cells (E PDCs) in development, cardiac disease and repair of ischemia. J Cell Mol Med.2010; 14: 1056–60.
25.
Rupp H, Rupp TP, Alter P, et al .Intrapericardial procedures for cardiac regeneration by stem cells: need for mini-mal invasive access (AttachLifter) to the normal pericardial cavity. Herz . 2010; 35:458–65.
26.
Zhou J, Zhang Y, Wen X, et al .Telocytes accompanying cardiomyocyte in primary culture: two- and three-dimensional cul-ture environment. J Cell Mol Med . 2010;14: 2641–5.
27.
Li TS, Cheng K, Lee ST, et al .Cardiospheres recapitulate a niche-like microenvironment rich in stemness and cell-matrix interactions, rationalizing their enhanced functional potency for myocar-dial repair. Stem Cells . 2010; 28: 2088–98.28.
Klumpp D, Horch RE, Kneser U, et al .E ngineering skeletal muscle tissue – new perspectives in vitro and in vivo . J Cell MolMed . 2010; 14: 2622–9.
29.
Kostin S.Types of cardiomyocyte death and clinical outcomes in patients with heart failure. J Am Coll Cardiol . 2011; 57:1532–4.
30.
Limana F, Capogrossi MC, Germani A.The epicardium in cardiac repair: from the stem cell view. Pharmacol Ther.2011; 129:82–96.
31.
Gard JJ, Asirvatham SJ.The “slow path-way” potential: fact or fiction? Circ Arrhythm Electrophysiol . 2011; 4: 125–7.32.
Russell JL, Goetsch SC, Gaiano N R, et al .A dynamic notch injury response activates epicardium and contributes to fibrosis repair. Circ Res . 2011; 108: 51–9.33.
Rusu MC, Pop F, Hostiuc S, et al .Extrahepatic and intrahepatic human portal interstitial Cajal cells. Anat Rec . 2011; 294:1382–92.
34.
Xiao J, Liang D, Chen YH.The genetics of atrial fibrillation: from the bench to the bedside. Annu Rev Genomics Hum Genet . 2011; doi: 10.1146/annurev-genom-082410-101515.
35.
Horst Ibelgaufts.Cytokines & Cells Online Pathfinder E ncyclopedia. 2011;https://www.wendangku.net/doc/453855004.html,/cope.cgi?key ?telocytes.
https://www.wendangku.net/doc/453855004.html,flamme MA, Murry CE.Heart regenera-tion. Nature . 2011; 473: 326–35.
37.
Liu JJ, Shen XT, Zheng X, et al .Distribution of telocytes in the rat heart. J Clin Rehabil Tiss Eng Res . 2011; 15: 3546–8.
38.
Od?rfer KI, Walter I, Kleiter M, et al .Role of endogenous bone marrow cells in long-term repair mechanisms after myocardial infarction. J Cell Mol Med . 2008; 12:2867–74.
39.
Mandache E, Gherghiceanu M, Macarie C, et al .Telocytes in human isolated atrial amyloidosis: ultrastructural remodelling. J Cell Mol Med.2010; 14: 2739–47.
40.Hinescu ME, Gherghiceanu M, Suciu
L, et al .Telocytes in pleura: two- and three-dimensional imaging by transmis-sion electron microscopy. Cell Tissue Res.2011; 343: 389–97.
41.Popescu LM, Gherghiceanu M, Suciu LC,
et al .Telocytes and putative stem cells in the lungs: electron microscopy, electron tomography, and laser scanning microscopy. Cell Tissue Res.2011; doi:10.1007/s00441-011-1229-z.
42.Suciu L, Popescu LM, Gherghiceanu M,
et al .Telocytes in human term placenta:morphology and phenotype. Cells Tissues Organs.2010; 192: 325–39.
43.Popescu LM, Manole E, Serboiu CS,
et al .Identification of telocytes in skeletal muscle interstitium: implication for muscle regeneration. J Cell Mol Med.2011; 15:1379–92.
44.Cismasiu VB, Radu E, Popescu LM.miR-193 expression differentiates telocytes from other stromal cells. J Cell Mol Med.2011; 15: 1071–4.
45.Popescu LM, Gherghiceanu M, Hinescu
ME, et al .Insights into the interstitium of ventricular myocardium: interstitial Cajal-like cells (ICLC). J Cell Mol Med . 2006; 10:429–58.
46.Eyden B.The myofibroblast: phenotypic
characterization as a prerequisite to under-standing its functions in translational med-icine. J Cell Mol Med . 2008; 12: 22–37.47.Schurch W, Seemayer TA, Gabbiani G.
The myofibroblast: a quarter century after its discovery. Am J Surg Pathol . 1998; 22:141–7.
48.Eyden B.The myofibroblast: an assess-ment of controversial issues and a defini-tion useful in diagnosis and research.Ultrastruct Pathol . 2001; 25: 39–50.
49.Eming SA, Hubbell JA.Extracellular
matrix in angiogenesis: dynamic struc-tures with translational potential. Exp Dermatol . 2011; 20: 605–13.
50.Lupu M, Khalil M, Iordache F, et al .
Direct contact of umbilical cord blood endothelial progenitors with living cardiac tissue is a requirement for vascular tube-like structures formation. J Cell Mol Med .2011; 15: 1914–26.
51.Zhao T, Zhao W, Chen Y, et al .Vascular
endothelial growth factor (VE GF)-A: role on cardiac angiogenesis following myocar-dial infarction. Microvasc Res . 2010; 80:188–94.
52.Gherghiceanu M, Popescu LM.Heterocellular
communication in the heart: electron tomography of telocyte-myocyte junc-tions. J Cell Mol Med . 2011; 15: 1005–11.
2296
? 2011 The Authors
Journal of Cellular and Molecular Medicine ? 2011 Foundation for Cellular and Molecular Medicine/Blackwell Publishing Ltd
53.Rana S, Z?ller M.E xosome target cell
selection and the importance of exosomal tetraspanins: a hypothesis. Biochem Soc Trans . 2011; 39: 559–62.
54.Martinez MC, Andriantsitohaina R.
Microparticles in angiogenesis: therapeutic potential. Circ Res . 2011; 109: 110–9.
55.Record M, Subra C, Silvente-Poirot
S, et al .xosomes as intercellular signalosomes and pharmacological effec-tors. Biochem Pharmacol . 2011; 81:1171–82.
56.Sen CK.MicroRNAs as new maestro
conducting the expanding symphony orchestra of regenerative and reparative medicine. Physiol Genomics . 2011; 43:517–20.
57.Wang S, Aurora AB, Johnson BA, et al .
The endothelial-specific microRNA miR-126 governs vascular integrity and angio-genesis. Dev Cell . 2008; 15: 261–71.
58.Chen Y, Gorski DH.Regulation of angio-genesis through a microRNA (miR-130a)that down-regulates antiangiogenic home-obox genes GAX and HOXA5. Blood . 2008;111: 1217–26.
59.Kuehbacher A, Urbich C, Zeiher AM,
et al .Role of Dicer and Drosha for endothelial microRNA expression and angiogenesis. Circ Res . 2007; 101: 59–68.60.Otsuka M, Zheng M, Hayashi M,
et al .Impaired microRNA processing causes corpus luteum insufficiency and
infertility in mice. J Clin Invest . 2008; 118:1944–54.
61.
Shen X, Fang J, Lv X, et al .Heparin impairs angiogenesis through inhibition of MicroRNA-10b. J Biol Chem . 2011; 286:26616–27.
62.
Urbich C, Kuehbacher A, Dimmeler S.Role of microRNAs in vascular diseases,inflammation, and angiogenesis. Cardiovasc Res . 2008; 79: 581–8.
63.
Caporali A, Meloni M, V?llenkle C, et al .Deregulation of microRNA-503 contributes to diabetes mellitus-induced impairment of endothelial function and reparative angio-genesis after limb ischemia. Circulation .2011; 123: 282–91.
64.
Liu LZ, Li C, Chen Q, et al .MiR-21induced angiogenesis through AKT and E RK activation and HIF-1?expression.PLoS One . 2011; 6: e19139.
65.
Zhou Q, Gallagher R, Ufret-Vincenty R,et al .Regulation of angiogenesis and choroidal neovascularization by members of microRNA-23~27~24 clusters. Proc Natl Acad Sci USA . 2011; 108: 8287–92.66.
Grundmann S, Hans FP , Kinniry S, et al .MicroRNA-100 regulates neovasculariza-tion by suppression of mammalian target of rapamycin in endothelial and vascular smooth muscle cells. Circulation . 2011;123: 999–1009.
67.
Elia L, Quintavalle M, Zhang J, et al .The knockout of miR-143 and -145 alters
smooth muscle cell maintenance and vascu-lar homeostasis in mice: correlates with human disease. Cell Death Diff.2009; 16:1590–8.
68.
Ferrara N, Davis-Smyth T.The biology of vascular endothelial growth factor. Endocr Rev.1997; 18: 4–25.
69.
N eufeld G, Cohen T, Gengrinovitch S, et al .Vascular endothelial growth factor (VEGF) and its receptors. FASEB J.1999;13: 9–22.
70.
Morbidelli L, Chang CH, Douglas JG, et al .Nitric oxide mediates mitogenic effect of VEGF on coronary venular endothelium.Am J Physiol.1996; 270: H411–5.
71.
Murohara T, Asahara T, Silver M, et al .Nitric oxide synthase modulates angiogen-esis in response to tissue ischemia . J Clin Invest.1998; 101: 2567–78.
72.
Kumar AH, Caplice N M.Clinical poten-tial of adult vascular progenitor cells.Arterioscler Thromb Vasc Biol.2010; 30:1080–7.
73.
Sahoo S, Klychko E, Thorne T,et al.Exosomes from human CD34+ stem cells mediate their proangiogenic paracrine activity. Circ Res.2011; 109: 724–8. 74.
Senger DR, Davis GE.Angiogenesis. Cold Spring Harb Perspect Biol.2011; 3: pii:a005090.
75.
Ribatti D, Nico B, Crivellato E.The role of pericytes in angiogenesis. Int J Dev Biol.2011; 55: 261–8.