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Ann Thorac Surg 1996;62:654-660
© 1996 The Society of Thoracic Surgeons

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Original Articles: Cardiovascular

Cardiomyocyte Transplantation Improves Heart Function

Division of Cardiovascular Surgery, Department of Clinical Biochemistry, and The Centre for Cardiovascular Research, The Toronto Hospital-General Division, University of Toronto, Toronto, Ontario, Canada

	Abstract

Top Footnotes Abstract Introduction Material and Methods Results Comment Acknowledgments References

 
Background. Transplantation of cultured cardiomyocytes into myocardial scar tissue may prevent heart failure.

Methods. Scar tissue was produced in the left ventricular free wall of 15 rats (weight, 450 g) by cryoinjury. Seven animals had operation only and survived for 8 weeks (sham group). Four weeks after cryoinjury, cultured fetal rat cardiomyocytes or culture medium was injected into the scar tissue of transplantation (n = 5) and control (n = 5) animals, respectively. Five other rats were sacrificed for scar assessment. Eight weeks after cryoinjury heart function in the transplantation, control, and sham groups was measured using a Langendorff preparation. Histologic studies were performed to quantify the extent of the scar and the transplanted cells.

Results. Four weeks after cryoinjury, 36% ± 4% (mean ± 1 standard error) of the left ventricular free wall surface area was scar tissue. At 8 weeks, the scar size had increased (p < 0.01) to 55% ± 3% in the control group. Although the scar size (43% ± 2%) in the transplantation group at 8 weeks was not significantly different from that at 4 weeks, it was less (p < 0.05) than that in the control group. Hearts in the sham group had no scar tissue. The transplanted cardiomyocytes had formed cardiac tissue within the myocardial scar. Systolic and developed pressures in the transplantation group hearts were greater (p = 0.0001) than in the control group hearts but less (p < 0.01) than those in the sham group hearts.

Conclusions. The transplanted cardiomyocytes formed cardiac tissue in the myocardial scar, limited scar expansion, and improved heart function compared with findings in the control hearts.

	Introduction

Top Footnotes Abstract Introduction Material and Methods Results Comment Acknowledgments References

 
See also page 660.

After a myocardial infarction, the damaged cardiomyocytes are gradually replaced by fibrous tissue with loss of regional contractile function. Ventricular remodeling results in wall thinning, which can cause aneurysm formation [1]. Heart failure may develop. The myocardial dysfunction is primarily due to the loss of cardiomyocytes. Cardiomyocyte transplantation into the ventricular scar offers the hope of restoring some ventricular function.

Transplanted cardiomyocytes have been shown to survive, proliferate, and connect with the host murine myocardium [2, 3]. We [4] demonstrated that fetal rat cardiomyocytes transplanted into the subcutaneous tissue of the adult rat leg formed cardiac tissue that contracted for the 3-month duration of the study. We have also shown that transplanted cardiomyocytes can survive in a rat myocardial scar (unpublished observation). To determine whether cardiomyocyte transplantation prevents heart failure, we transplanted fetal rat cardiomyocytes into scar tissue of the cryonecrosed left ventricular free wall (LVFW) of adult rat hearts. The transplanted cardiomyocytes limited the expansion of scar tissue and improved heart function.

	Material and Methods

Top Footnotes Abstract Introduction Material and Methods Results Comment Acknowledgments References

 
Experimental Animals
All procedures performed on animals were approved by the Animal Care Committee of The Toronto Hospital. Experimental animals used were Sprague-Dawley rats (Lewis; Charles River Canada Inc, Quebec, PQ, Canada). Twenty-two male rats weighing 400 to 450 g served as recipients. Cardiomyocytes obtained from 18-day gestational rat hearts were cultured prior to transplantation. All experiments were performed according to the "Guide to the Care and Use of Experimental Animals" of the Canadian Council on Animal Care and the "Guide for the Care and Use of Laboratory Animals" published by the National Institutes of Health (NIH publication 85-23, revised 1985).

Cell Culture and Preparation for Transplantation
Cardiomyocytes from fetal rat hearts were isolated, purified, and cultured as previously described [4, 5]. The purified cardiomyocytes were transfected by the calcium phosphate coprecipitation technique [6] with pRSV-lacZ plasmid containing ß-galactosidase gene (a generous gift of Dr R. Chiu, Montreal General Hospital, Montreal, PQ, Canada) for identification of the transplanted cells in the myocardial scar tissue. Cultures of the cells were grown for 24 hours in Iscove's modified Dulbecco's medium containing 10% fetal bovine serum, 100 U/mL of penicillin, and 100 ug/mL of streptomycin at 37°C in 5% carbon dioxide and 95% air. The transfected cardiomyocytes were detached from the cell culture dish with 0.05% trypsin in phosphate-buffered saline solution. After centrifugation at 580 g for 3 minutes, the cell pellet was resuspended in culture medium at a concentration of 16 x 10⁶ cells/mL. A 0.25-mL cell suspension was used for each transplantation.

Anesthesia and Postoperative Care of Rats
Adult rats were anesthetized with intramuscular administration of ketamine hydrochloride (22 mg/kg) followed by an intraperitoneal injection of sodium pentobarbital (30 mg/kg). The anesthetized rats were intubated, and positive-pressure ventilation was maintained with room air supplemented with oxygen (6 L/min) using a Harvard ventilator (model 683). The rats were monitored for 4 hours postoperatively. Penlong XL (penicillin G benzathine, 150,000 U/mL, and penicillin G procaine, 150,000 U/mL) was given intramuscularly (0.25 mL per rat) every 3 days for 1 week after operation, and buprenorphine hydrochloride (0.01 to 0.05 mg/kg) was administered subcutaneously every 8 to 12 hours for the first 48 hours after operation.

Myocardial Scar Formation
Under general anesthesia, the adult rat heart was exposed through a 2-cm left lateral thoracotomy. For the animals having a sham operation (sham group) (n = 7), the surgical incision was then closed with 5-0 Vicryl sutures. Cryoinjury was produced in 15 animals with a metal probe 8 x 10 mm in diameter cooled to -190°C by immersion in liquid nitrogen and then applied to the LVFW for 1 minute. This procedure was repeated four times. The muscle layer and the skin incision were then closed with 5-0 Vicryl sutures. Antibiotics and analgesics were given as already described. The 15 cryoinjured animals were randomly divided into three equal groups: pretransplantation, control, and transplantation.

Cardiomyocyte Transplantation
Four weeks after cryoinjury, the pretransplantation hearts (n = 5) were harvested for histologic and planimetric studies. Under general anesthesia, the hearts in the control (n = 5) and transplantation (n = 5) groups were exposed through a midline sternotomy. A fetal rat cardiomyocyte suspension (0.25 mL, 4 x 10⁶ cells) was injected once into the center of the scar tissue in the transplantation group using a tuberculin syringe, and 0.25 mL of cell culture medium was injected into the scar tissue in the control group. The chest was closed with 5-0 Vicryl sutures. The rats in the sham group (n = 7) underwent the same procedure without injection. Antibiotics and analgesics were given as previously described. Cyclosporin A, 5 mg • kg^-1 • d^-1, was administered subcutaneously to the control and transplantation groups. The rats were housed in cages with filter tops.

Myocardial Function Studies
Eight weeks after cryoinjury, heart function in the sham, control, and transplantation groups was measured using a Langendorff preparation [7]. The rats were anesthetized, and heparin sodium (200 units) was administered intravenously. The hearts were quickly isolated and perfused in a Langendorff apparatus with filtered Krebs-Henseleit buffer (mmol/L:NaCl, 118; KCl, 4.7; KH₂PO₄, 1.2; CaCl₂, 2.5; MgSO₄, 1.2; NaHCO₃, 25; and glucose, 11; pH 7.4) equilibrated with 5% carbon dioxide and 95% oxygen. A latex balloon was passed into the left ventricle through the mitral valve and connected to a pressure transducer (model p10EZ; Viggo-Spectramed, Oxnard, CA) and a transducer amplifier and differentiator amplifier (model 11-G4113-01; Gould Instrument System Inc, Valley View, OH).

After 30 minutes of stabilization, the coronary flow of the heart was measured in triplicate by timed collection in the empty beating state. The balloon size was increased in 0.02-mL increments from 0.04 to 0.46 mL by the addition of saline solution. The systolic and diastolic pressures were recorded at each balloon volume, and developed pressure was calculated as the difference between the systolic and diastolic pressures.

The heart was weighed and the size measured by water displacement.

Measurement of LVFW Remodeling
The epicardial and endocardial surface areas of the normal and scar tissue in the LVFW were measured by the techniques of Pfeffer and associates [8] and Jugdutt and Khan [9]. Briefly, the hearts were fixed in distention (30 mm Hg) with 10% phosphate-buffered formalin solution and then cut into sections 3 mm thick. For each section, the areas of normal tissue, scar tissue, and transplanted tissue in the LVFW were traced onto a transparency and quantified using computed planimetry (Jandal Scientific Sigma-Scan, Corte Madera, CA). The lengths of the LVFW and the scar tissue on both the endocardial and epicardial surfaces of each section were measured. The surface areas of the epicardial and endocardial scar tissue and the LVFW were measured as the sum of the endocardial length and epicardial length times the section thickness (3 mm). The surface area percentage of scar tissue in the LVFW was calculated as follows:

To calculate the percentage of the surface area in the scar tissue occupied by "cardiac tissue," the cardiac tissue length in the scar tissue of each section times the section thickness (3 mm) was added and then divided by the total scar area times 100.

Histologic Studies
The heart sections were fixed in 5% glacial acetic acid in methanol, embedded in paraffin, and sectioned to yield slices 10 µm thick. The slices were stained with hematoxylin and eosin as described in the manufacturer's specifications (Sigma Diagnostics, St. Louis, MO).

To stain for in vitro ß-galactosidase activity in the cultured fetal cardiomyocytes, the cells were washed three times with phosphate-buffered saline solution and fixed in 2% formaldehyde and 2% glutaraldehyde in phosphate buffer (0.15 mol/L NaCl and 0.015 mol/L NaH₂PO₄; pH 7.2) at 4°C for 5 minutes. After washing with phosphate buffer containing 2.0 mmol/L MgCl₂, the cells were stained overnight at 37°C in a solution containing 1 mg/mL of 5-bromo-4-chloro-3-indolyl-beta-galactopyranoside (X-gal), 5 mmol/L K₃Fe(CN)₆, 5 mmol/L K₄Fe(CN)₆•3H₂O, and 0.2 mmol/L MgCl₂ in phosphate buffer (pH 7.2). The stained and nonstained cells (100 cells per dish) in six dishes were counted under a microscope to determine the percentage of cells containing ß-galactosidase activity.

To stain for ß-galactosidase activity in the transplanted cardiomyocytes, the heart sections were fixed in 2% formaldehyde and 2% glutaraldehyde in phosphate buffer at 4°C for 12 hours. The tissue was then stained for ß-galactosidase activity at 37°C for 24 hours as just described. The heart section was embedded in paraffin and sectioned to yield slices 10 µm thick. After removal of the paraffin using xylene and followed by clearing in 100%-95%-90%-85%-70% ethanol (3 minutes each), the stained cells were photographed.

Data Analysis
Data are expressed as the mean ± the standard error. Statistical Analysis System software was used for all analyses (SAS Institute, Cary, NC). Comparisons of continuous variables between more than two groups were performed by a one-way analysis of variance. If the F ratio was significant from the analysis of variance, a Duncan's multiple-range t test was employed to specify differences between groups. The critical -level for these analyses was set at a p value of less than 0.05.

Functional data were evaluated for the sham, control, and transplantation groups by an analysis of covariance using intracavitary balloon volume as the covariant-factor and systolic, diastolic, and developed pressures as dependent variables. Main effects were group, volume, and interaction between group x volume. If there was an overall difference in the analysis of covariance, multiple pairwise comparisons were performed to specify which groups were different. Because there were multiple pairwise comparisons, a Bonferroni correction was performed, and the critical level was set at 0.01 for the analysis of covariance.

	Results

Top Footnotes Abstract Introduction Material and Methods Results Comment Acknowledgments References

 
The fetal rat cardiomyocytes were isolated and cultured. The viable cells attached to the culture dish within 4 hours after purification. The cells contracted regularly and spontaneously. The ß-galactosidase transfecting efficiency of the cultured cardiomyocytes was 21% ± 4% (n = 6).

Four weeks after transplantation, the fetal cells had formed cardiac tissue in the myocardial scar tissue of the transplantation group (n = 5) (Figs 1, 2). The transplanted cells stained positively for ß-galactosidase activity (see Fig 2a). The cells were elongated, contained organized sarcomeres, and were connected to each other by intercalated discs (Fig 3; see Figs 2b, 2c). Blood vessels were present in the transplanted tissue, and lymphocytes surrounded it. There was no cardiac tissue in the myocardial scar of the control animals (n = 5) (Fig 4; see Fig 1). The sham group had no LVFW scar tissue.

View larger version (27K): [in this window] [in a new window]   Fig 1. . Photographs of adult rat hearts from transplantation and control groups 8 weeks after cryoinjury. (a, b) The size of the left ventricular free wall (LVFW) and transmural scar tissue (short arrows) in the control heart is larger and thinner than that of the transplantation heart. The transplanted cardiomyocytes formed tissue in the LVFW (long arrows).

View larger version (42K): [in this window] [in a new window]   Fig 2. . Photomicrographs of fetal rat cardiomyocytes 4 weeks after transplantation into myocardial scar. (a) Transplanted cardiomyocytes stained for ß-galactosidase activity. (b) Transplanted cardiac tissue (TM) in myocardial scar tissue (S). (c) Transplanted cardiac tissue showing striated cardiomyocytes (TM), lymphocytes (L), and a scar (S). Arrows point at blood vessels. (b, c: hematoxylin and eosin; a, c: x200 before 46% reduction; b: x40 before 46% reduction.) (M = normal myocardium.)

View larger version (88K): [in this window] [in a new window]   Fig 3. . Electron micrograph of transplanted cardiomyocytes in myocardial scar tissue. Arrows point at intercalated discs. (x2,600 before 50% reduction.) (S = sarcomere.)

View larger version (32K): [in this window] [in a new window]   Fig 4. . (a, b) Scar tissue (S) formed in left ventricular free wall of control rat heart 8 weeks after cryoinjury. (Both: hematoxylin and eosin; a, x40 before 46% reduction; b, x200 before 46% reduction.) (M = normal myocardium.)

View larger version (18K): [in this window] [in a new window]   Fig 5. . Surface area percentages of scar tissue in left ventricular free wall (LVFW) for pretransplantation group 4 weeks after cryoinjury, control group 8 weeks after cryoinjury, and transplantation group 8 weeks after cryoinjury. The transplanted cells occupied 37% of the scar in the LVFW. (**p < 0.01; *p < 0.05.)

View larger version (41K): [in this window] [in a new window]   Fig 6. . Developed, systolic, and diastolic pressures of sham, control, and transplantation group hearts with increasing balloon volumes. Systolic and developed pressures in the transplantation group were significantly higher than those of the control group (both, p = 0.0001) but lower than those of the sham group (both, p = 0.0001).

View larger version (23K): [in this window] [in a new window]   Fig 7. . Developed pressures of sham, control, and transplantation group hearts at balloon volumes of 0.1 and 0.2 mL. Developed pressure in the transplantation group was significantly higher than in the control group but lower than in the sham group by analysis of covariance at both balloon volumes. (*p < 0.01; a versus b, p < 0.01)

	Comment

Top Footnotes Abstract Introduction Material and Methods Results Comment Acknowledgments References

Transplantation of cultured cardiomyocytes is a possible technique of replacing scar tissue. Koh and associates [2] transplanted AT-1 cardiomyocytes (a cell line isolated from subcutaneous tumors derived from the left atrium of transgenic mice) into syngeneic mouse hearts and found that the transplanted cells survived and proliferated. Angiogenesis occurred in the transplant [10]. The same research group [3] found that the transplanted cardiomyocytes survived and formed gap junctions with host cardiomyocytes in the host myocardium. Because the clinical application of cardiomyocyte transplantation requires the transplanted cells to survive and function in fibrous tissue (myocardial scar tissue), we extended these observations. In previous studies, we [4] found that fetal rat cardiomyocytes transplanted into the subcutaneous tissue of the adult rat leg were viable and formed cardiac tissue, which contracted for the 3-month duration of the experiment. When fetal cardiomyocytes were transplanted into a homogeneous scar in adult rat hearts, the transplanted cells survived and formed cardiac tissue for the 2-month duration of the study (unpublished observations).

Coronary artery ligation is often used experimentally to produce a myocardial infarction and scar tissue. However, coronary ligation produces a wide spectrum of necrosis, scar tissue, and ventricular dysfunction in rats [8]. The extent and homogeneity of the scar is dependent on the amount of collateral perfusion, which is variable [11]. Although myocardial necrosis and scar formation resulting from cryoinjury are not clinically relevant, the transmural scar is more constant in size and myocardial dysfunction is less variable than seen after coronary ligation. In the present study cryoinjury generated a homogeneous scar occupying 36% ± 4% of the LVFW at 4 weeks and 55% ± 3% at 8 weeks. However, experiments using an animal model of myocardial infarction produced by coronary artery ligation will be necessary to determine whether our results have clinical relevance.

Four weeks after cryoinjury, a maturing scar was present. Fetal rat cardiomyocytes were transplanted at 4 weeks to avoid the inflammatory reaction that occurs in the ventricular wall immediately after cryoinjury. Four weeks after transplantation, the transplanted cardiomyocytes had survived and formed a cardiac tissue that stained positive for ß-galactosidase activity. The arrangement of the cardiomyocytes appeared to be disorganized compared with the arrangement in the host cells. The transplanted cells were connected to each other by intercalated discs. The tissue was more vascular than surrounding scar tissue. The presence of lymphocytes indicated rejection of the transplant despite cyclosporine treatment. The relative importance of cardiomyocyte hypertrophy and hyperplasia in forming the transplant in the scar is unknown.

The explanation for improved heart function by cardiomyocyte transplantation was not determined in this study. Cardiomyocyte transplantation limited scar thinning and expansion. The smaller ventricle prevented overstretching of the host and transplanted cardiomyocytes, thus resulting in improved contractile force compared with control hearts. Four mechanisms are possible: (1) cardiomyocyte contractility; (2) cardiomyocyte elastic properties; (3) revascularization; and (4) a factor secreted by the transplanted cardiomyocytes. The transplanted tissue was contractile and occupied 37% of the scar. The transplanted tissue was unlikely to contract synchronously with the host myocardium because the cells were injected into the center of the scar and did not appear to be in contact with the host cardiomyocytes. Although the contribution of the transplant contractility to overall function is unknown, it was modest. Another possible mechanism of the beneficial effect of cardiomyocyte transplantation is the elastic properties of the contractile apparatus of the transplanted cardiomyocytes. These properties would prevent fibroblast stretching and ventricular enlargement. With each ventricular contraction, the elastic properties may have tended to restore the ventricular wall to its original size and shape. The development of angiogenesis may also have limited scar expansion and modified ventricular remodeling [12]. The increased blood supply in the scar may have facilitated fibroblast turnover and strengthening of the scar in response to ventricular stretch. Finally, the transplanted cardiomyocytes could secrete a factor that stimulates fibroblast turnover and prevents scar thinning and expansion.

Cardiomyocyte transplantation may have clinical applications. Transplantation early after an infarction at the time of coronary artery bypass grafting to treat persistent angina could prevent scar expansion, restore contractility of the infarcted region, and reduce the long-term morbidity and mortality after surgical revascularization. Late after a myocardial infarction, contractility could be restored by resecting the thin scar and reconstructing the normal geometry with a pericardial patch [13]. Cardiomyocytes could be placed on a pericardial patch used to reconstruct the ventricle. If the transplanted cardiomyocytes developed into contracting tissue that formed junctions with the host myocardium and contracted synchronously, cardiac function might be restored. A cardiac pacemaker would be required if the transplant did not beat synchronously with the heart.

Although human fetal cardiomyocytes could be transplanted into the infarcted heart, patients would require immunosuppressants to prevent rejection. We [14–16] have grown human cardiomyocytes from myocardial specimens obtained from children and adults undergoing cardiac operations. However, these cardiomyocytes did not beat spontaneously even though the cultured cells contained contractile proteins such as human ventricular myosin heavy chain, light chain, cardiac-specific troponin I isoform, T, and actin. If these inactive cardiomyocytes could be induced to contract, they could be used for transplantation.

Simpson and co-workers [17] found that exposing cardiomyocytes to mechanical stimuli could induce alignment of the contractile apparatus. In a pilot study, we transfected human pediatric cardiomyocytes with a plasmid containing ß-galactosidase gene and cultured them on top of confluent beating fetal rat cardiomyocytes. After 5 days, the cultured cells beat synchronously. Electron microscopy showed transfected human cardiomyocytes contained crystalloid inclusions produced by ß-galactosidase, and many myofilaments were lined up in the cytoplasm. If future research can develop the technology to stimulate the transplanted cardiomyocytes to reform their sarcomeres and to induce angiogenesis, ventricular cardiomyocytes obtained from transvenous endocardial specimens could be grown and autotransplantation could become a reality. The transplanted cells should form intercalated junctions with the host cardiomyocytes, beat synchronously, and improve infarcted heart function.

	Acknowledgments

Top Footnotes Abstract Introduction Material and Methods Results Comment Acknowledgments References

 
This study was supported by the Heart and Stroke Foundation of Ontario (grant A2604) and the Medical Research Council of Canada (grant MT-10392).

We thank Judy Birth for assistance in the fetal rat heart preparation, Dr Guang Ming Li for help in the histologic examination, and Dr Frank Merante for cell transfection.

	Footnotes

Top Footnotes Abstract Introduction Material and Methods Results Comment Acknowledgments References

 
Presented at the Thirty-second Annual Meeting of The Society of Thoracic Surgeons, Orlando, FL, Jan 29–31, 1996.

Address reprint requests to Dr Li, Toronto Hospital-General Division, CCRW 1-854, 200 Elizabeth St, Toronto, Ont, Canada M5G 2C4.

	References

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3. Soonpaa MH, Koh GY, Klug MG, Field LJ. Formation of nascent intercalated disks between grafted fetal cardiomyocytes and host myocardium. Science 1994;264:98–101.[Abstract/Free Full Text]
4. Li R-K, Mickle DAG, Weisel RD, Zhang J, Mohabeer MK. In vivo survival and function of transplanted rat cardiomyocytes. Circ Res 1996;78:283–8.[Abstract/Free Full Text]
5. Mickle DAG, Li R-K, Weisel RD, et al. Myocardial salvage with Trolox and ascorbic acid for an acute evolving infarction. Ann Thorac Surg 1989;47:553–7.
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10. Koh GY, Kim SJ, Klug MG, Park K, Soonpaa MH, Field LJ. Targeted expression of transforming growth factor-ß1 in intracardiac grafts promotes vascular endothelial cell DNA synthesis. J Clin Invest 1995;95:114–21.
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15. Li R-K, Shaikh N, Weisel RD, Williams WG, Mickle DAG. Oxyradical-induced antioxidant and lipid changes in cultured human cardiomyocytes. Am J Physiol 1994;266(Heart Circ Physiol 35):H2204–11.[Abstract/Free Full Text]
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