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Effect of uremia on incorporation of acetate into rat plasma and tissue lipids
Effect of Uremia on Incorporation and Tissue Robert
J. Morin,
Mayasandra
U
REMIA results in a hyperlipidemic state in man and animals’,2 and may be a major cause of the increased atherosclerosis and its complications observed in chronic renal disease patients.3’4 The hyperlipidemias and atherosclerosis have been reported in some studies to be worse in renal disease patients undergoing hemodialysis than in those not receiving this treatmenL4” Acetate is the most common alkalinizing agent used during hemodialysis, and these patients are subjected to large unphysiologic plasma acetate loads.6S7 Acetate is a well known lipid precursor, which might contribute to the elevated plasma lipids in these patients. The present investigation was aimed at determining whether experimental uremia alters either the catabolism of acetate to CO, or its conversion to plasma and tissue lipids, so as to gain further insight into the possible aggravating factors in uremic hyperlipidemia. AND
METHODS
Sixty male Sprague-Dawley rats weighing about 200 g were used in this study, and were divided into six groups containing IO rats each. The groups were: (1) sham operated-studied 0.5 hr after operation; (2) bilateral nephrecMetsbolism,
Vol.
29,
No.
4
(April),
1980
Into Rat Plasma
Lipids
V. Srikantaiah.
Experimental uremia was induced in rats by means of bilateral nephrectomy or bilateral ureteral ligation. Incorporation of acetate-l -‘k into expired ‘*CO2 and into plasma and tissue lipids was studied immediately after surgery and at 48 hr, when the rats were uremic. In rats studied immediately after surgery, bilateral nephrectomy. but not bilateral ureteral ligation. significantly decreased the conversion of acetate-l-‘? into expired ‘%O,. In uremic rats at 48 hr. acetate-l -‘% metabolism to “CO, was not significantly altered in either group. Plasma triglyceride concentrations and ‘%-acetate incorporation into triglycerides were increased in the 48-hr uremic groups, but plasma and liver triglyceride specific radioactivities were not significantly altered. Plasma free fatty acid concentrations and incorporation of acetate into free fatty acids were lower in the 48-hr uremic groups than in controls. Plasma cholesterol concentrations and specific radioactivities were increased in these uremic groups, as were liver free cholesterol specific activities. These results suggest that increased triglyceride and cholesterol synthesis from acetate may contribute to the hypertriglyceridemia and hypercholesterolemia observed in uremic rats.
MATERIALS
of Acetate and Warren
D. Davidson
tomy (renal artery ligation)-studied 0.5 hr after ligation: (3) bilateral ureteral ligation-studied 0.5 hr after ligation; (4) sham operated-studied 48 hr after operation; (5) bilateral nephrectomy-studied 48 hr after nephrectomy; and (6) bilateral ureteral ligation-studied 48 hr after ligation. The rats were maintained in the fasting state and then were given acetate-l-‘% (59.0 mCi/mmol. New England Nuclear. Boston, Mass.), 100 &i/kg and nonradioactive acetate, 10 mmole/kg intraperitoneally. “C0Z in expired air from each rat was monitored continuously for 4 hr using a vibrating reed electrometer-ionization chamber method.’ The rats were killed by exsanguination and blood and tissues were obtained for lipid analysis. Total lipids in rat plasma, liver, epididymal adipose tissue, aorta, spleen. testes, and kidney were extracted by homogenization twice in 10 times their volume of chloroform/ methanol, 2/ 1. using a Polytron homogenizer. The combined extracts were washed with acetate buffer (pH 4.0) to remove nonlipid components. Mean recovery of total lipids was 94%. Phospholipid concentrations were determined following digestion of aliquots of the washed lipid extracts at 180°C for 2.5 hr with perchloric acid. Calorimetric phosphate analysis was done by addition of hydrazine sulfate. stannous chloride. and sodium molybdate, and optical densities at 815 nm recorded automatically using a Technicon Autoanalyzcr.’ Plasma triglycerides were extracted into N-nonane and isopropanol (2:3.5, volume:volume). After transesterification with ethoxide, free glycerol was recovered in the aqueous phase and color developed with acetylacetone.‘” The absorbance was read at 410 nm in a Hitachi spectrophotometer. Total plasma cholesterol was determined enzymatically.” In this method, serum cholesterol esters were hydrolyzed to free cholesterol by cholesterol ester hydrolase. The free cholesterol was then oxidized by cholesterol oxidase to cholest4-en-3-one, with the simultaneous production of hydrogen peroxide; the latter oxidatively couples with 4-amino antipyrine and phenol in the presence of peroxidase to yield a chromogen with maximum absorption at 500 nm A single aqueous reagent obtained from Abbott Laboratories. Chicago, Illinois was utilized, and after a IO-min incubation, optical densities were recorded automatically using an Abbott Bichromatic analyzer. Plasma free cholesterol was determined by the same method except that addition of _ From the Departments of Pathology and Medicine, Harbor General Hospital, UCLA School o/ Medicine. Torrance, Calif. Received for publication May 7. 1979. Supported by Artificial Kidney Program (NIH) Contract NOI-AM-S-2209 and NIH Training Grant AM-05383. Address reprint requests to Dr. Robert J. Morin, Department of Pathology. Harbor General Hospital, UCLA School of Medicine, 1000 West Carson Street, Torrance. Calif. 90509. 0 I980 by Grune & Stratton, Inc. 0026-0495/80/2904~003$01.00/0
311
312
MORIN.
SRIKANTAIAH,
AND DAVIDSON
cholesterol ester hydrolase was omitted. Plasma free fatty acids were determined calorimetrically after reaction of cobalt soaps of the free fatty acids with LYnitroso$ naphthol.” For determinations of radioactivities, plasma and liver lipid classes were separated by thin-layer chromatography on silica gel G plates coated with fluorescein. The plates were developed with petroleum ether-diethyl ether-acetic acid (SO:ZO: I), the lipid zones detected under UV light, collected, eluted, and radioactivities in aliquots of these eluates determined by lipid scintillation counting. Mean recovery of lipids was 90.5%. Significance of apparent differences between groups was determined by the t test for unpaired groups. RESULTS
The blood urea nitrogen levels in each of the experimental groups were as follows: sham (OShr), 24.6 mg/dl i 6.7 (SD); bilateral nephrectomy (0.5-hr), 52.9 f 11.6; bilateral ureteral ligation (0.5hr), 38.3 + 9.3; sham (48 hr), 20.8 + 3.8; bilateral nephrectomy (48 hr), 216.5 + 37.6; bilateral ureteral ligation (48 hr), 259.2 + 44.8. The time courses of oxidation of the administered 14C-acetate to “C0, in each of the experimental groups are indicated in Figs. 1 and 2. Percentages of the administered acetate catabolized to CO, over the 4-hr experimental period are shown in Table 1. In rats studied immediately after surgery (mild uremic groups), bilat-
MINUTES Fig. 2. Recovery of “CO, in expired air following intraperitoneal injection of acetate-l-? into uremic rats 48 hr after bilateral ureteral ligation (O---O) or bilateral nephrectomy (O---O) compared to sham operated. nonuremic controls (O---O). Each curve is the mean expired “CO, in 10 rats. The areas under the three curves (total recovery of “COJ are not significantly different.
era1 nephrectomy, but not bilateral ureteral ligation, significantly reduced the recovery of r4C0, from injected acetate-l-14C, compared with sham-operated controls. In the severely uremic rats, neither bilateral nephrectomy nor bilateral ureteral ligation significantly altered recovery of 14C0, from injected acetate- 1-14C, compared with sham operated or mild uremic controls. Results of rat plasma lipid analysis are indicated in Table 2. Free and esterified cholesterol and triglyceride concentrations were significantly elevated in the 4%hr nephrectomized and
ureteral ligation groups, whereas free fatty acids were decreased below the sham-operated controls in both these groups (p < 0.01 for all). As Table 1. “C0,
Recovery After
Acetate-l-‘?
Administration
ii Group
”
I%)
SD I%)
P
0.5-hr 0
30
60
90
120
I60
240
MINUTES Fig. 1. Recoveryof ‘*COz in expired air following intraperitoneal injection of acetate-l -‘*C into nonuremic rats 0.5 hr after bilateral ureteral ligation (O---O), bilateral nephrectomy (O--O), or sham operation (O--O). Each curve represents the mean expired ‘%ZO, in 10 rats. The area under the curve (i.e., recovery) for rats with bilateral nephrectomy is significantly less than in the sham operated rats. *Indicates p > 0.05 (see Table 1).
Sham
10
67.6
5.1
-
Bilateral nephrectomy
10
58.3
6.1
<0.0025*
Bilateral ureteral ligation
10
69.6 8.9
Sham
10
65.1
8.4
-
Bilateral nephrectomy
10
70.7
a.7
>o.o5t
Bilateral ureteral ligation
10
70.5
5.9
>o.o5t
>0.30’
48-hl
*Versus acute shams. tVersus chronic shams.
UREMIA
AND
LIPID
METABOLISM
313
Table 2. Plasma Lipid Concentrations
Group
in Control, Bilateral Nephrectomized.
Free
Esterified
Cholesterol
Cholesterol
and Bilateral Ureteral
TG
Ligated Rats
FFA
Phospholiplds
0.5hr
Sham
22.3
zk 1.1
49.3
2
1.9
25.8
+ 5.5
22.5
I
2.1
118.8
+ 6.1
Nephrectomy
20.7
r
1.5
51.6
f
2.6
24.4
+ 3.2
18.7
c
1.9
102.6
+ 7.0
Ureteral
27.9
+
1.7
52.2
+ 3.1
19.3
+ 2.0
22.3
+
1.3
90.0
5 6.7
Sham
25.6
k 0.8
57.9
+ 3.6
19.6
-i- 1.4
19.9
+
1.9
102.0
k 7.6
Nephrectomy
36.1
k 2.9’
75.1
t
5.5.
59.1
+ 7.2’
14.6
t
1.6*
137.6
+ 7.9
Ureteral
39.3
f
98.4
+ 7.2
50.1
r
15.0
t
2.0
109.0
i
ligation
48-hr
ligation
Abbreviations: Values
TG, triglycerides:
are mg/dl
*Indicates
48-hr
plasma
FFA,
3.0 free fatty
6.2
9.9
acids.
? SE.
nephrectomy
group
significantly
different
from
48-hr
sham,
seen in Table 3, acetate-14C incorporation into rat plasma total lipids was significantly increased in both the 48-hr nephrectomized and ureteral ligation groups compared with the 48-hr sham-operated group (p < 0.01). The percentage of total acetate-14C incorporated into free cholesterol, cholesterol esters, and triglycerides of the former two groups was increased, whereas the percentage incorporated into free fatty acids and phospholipids was decreased below that of Table 3. Incorporation
of Acetate-‘?
Total lbpid Group
p < 0.01
the 48-hr sham group (p < 0.01 for all). Similar results are seen when incorporation of acetate14C was calculated in terms of dpm incorporated into each of the individual plasma lipids/ml plasma. When calculated as specific radioactivity (Table 4, dpm/mg of each lipid class), only plasma free and esterified cholesterol showed an increased incorporation in the 48-hr nephrectomized and ureteral ligation groups compared with the 48-hr sham group (p < 0.01).
Into Plasma Total Lipids and Percent Distribution Free
Cholesterol
Cholesterol
Esters
1%)
(%I
(dpmlml)
in Lipid Classes
Free Fatty Tnglycerldes 1%)
Aads
Phospholipads
1%)
(%l
0.5-hr Sham
1084
k 59
9.2
k 0.6
20.8
k 0.9
27.8
+
1.4
3.3
i
0.2
40.3
1
Nephrectomy
1486
+
125
8.3
k 0.6
20.5
+
1.4
24.0
k 2.3
2.7
-r 0.2
44.2
+ 2.0
Ureteral
1025
f
64
9.9
*
24.8
t
1.4
20.2
+
1.4
2.9
i
0.4
42.6
i
2.5
ligation
0.5
1.6
2.2
48-hr Sham
i- 44
11.9
+ 0.9
23.5
f
13.3
k
1.1
2.9
+ 0.4
44.3
- 3.5
Nephrectomy
1943
739
+
153’
20.5
f
1.6*
37.4
+ 2.9s
22.5
+ 2.3’
1.0
f O.lf
20.5
-
1.8’
Ureteral
ligation
2225
-i
178’
21.3
+
1.7’
40.7
k 2.6*
24.4
k 3.1’
0.9
t
16.4
r
1.2’
that
nephrectomy
*Indicates
the 48-hr
and ureteral
Table 4.
Gr0Ul
ligation
groups
Specific Radioactivities
FrlX
Esterified
Cholesterol
Cholesterol
were
significantly
different
from
0.1
the 48-hr
l
sham
group.
p
I 0.01
of Individual Plasma Lipids
TG
FFA
Phosoholnds
0.5-hr Sham
494
+ 38
338
k 29
1145
-r 229
128
k
15
306
r
18
Nephrectomy
635
2 69
355
+ 38
1535
k 230
204
i
22
550
t
49
Ureteral
398
k 30
283
+ 17
1181
+
110
121
*
10
462
t
37
+ 22
ligation
48-hr Sham
38
189
+ 25
748
f
39
117
f
14
321
Nephrectomy
1184
341
-r 133*
659
+ 106’
752
t
90
121
*
14
325
i
Ureteral
1291
k
543+51*
913
*
109
110
+ 25
325
k 29
ligation
Abbreviations: Values
TG,
are dpm/mg
*Indicates
that
triglycerides: lipid
the 48-hr
FFA,
f
167* free fatty
22
acids.
+ SE. nephrectomy
and ureteral
ligation
groups
were
significantly
different
from
the 48-hr
sham
group.
p J_ 0.01.
314
MORIN,
Table 5. Liver Lipid Concentrations Free Cholesterol
GrOWI
in Control, Nephrectomized, Esterified Cholesterol
SRIKANTAIAH,
and Ureter-Ligated
TG
AND
DAVIDSON
Rats
Phospholipids
FFA
0.5hr Sham
0.8 k 0.05
1.8 r 0.12
7.8 r 0.8
1.02 + 0.42
31.0?
Nephrectomy
1.1 + 0.04
2.1 + 0.12
5.4 + 0.3
1.18 r 0.29
31.1
k 0.6
Ureteral ligation
1.1 + 0.08
1.9 ? 0.09
4.8 k 0.5
0.97
31.8
k 1.2
48-hr Sham
‘_ 0.09
0.8
0.9 + 0.03
2.0 + 0.18
4.5 f 0.5
0.47
c 0.05
30.0
i 0.7
Nephrectomy
0.8 f 0.04
1.8 f 0.10
10.5 + 1.5’
0.46
k 0.04
31.4
+ 0.6
Ureteral ligation
0.8 + 0.06
1.7 f 0.09
6.7 t 0.8
0.34
r 0.04
28.3
+ 0.8
Abbreviations: TG, triglycerides; FFA. free fatty acids. Values are mg/g wet wt liver f SE. *indicates that liver triglyceride concentration was significantly higher in the 48-hr nephrectomy group than in the 48-hr sham group, p < 0.01.
Liver lipid concentrations in these rat groups are given in Table 5. The only significant difference observed was an increase in triglyceride concentration in the 48-hr nephrectomized group compared with the 48-hr sham group (p < 0.01). Incorporation of acetate-i4C into liver total lipids (Table 6) was increased in the 48-hr nephrectomized and ureteral ligation groups compared with the 48-hr sham group (p < 0.01). The percentage of total acetate-14C activity incorporated into free cholesterol and triglycerides of the former two groups was increased, and the phospholipid fraction showed a decreased percentage of incorporation (p < 0.01 for both). Similar results were seen when incorporation was calculated as dpm in each lipid class/g liver, with the exception that incorporation into the phospholipids of the 48-hr nephrectomized group was not significantly different from the 48-hr sham group. As seen in Table 7, when calculated as dpm/mg lipid, only free cholesterol specific activity was higher in the 48-hr nephrecTable 6. Incorporation
Group 0.5hr Sham
DISCUSSION
The present results indicate that severe uremia in rats does not significantly alter the catabolism of acetate to C02, and that the observed differences in incorporation of acetate into plasma and tissue lipids are probably not attributable to differences in availability of substrate between the severe uremic and the control groups. Acetate pool size could not be measured, however, and our conclusions are based upon the assumption that these pool sizes remained the same in the groups compared. Plasma triglyceride levels were increased in
Into Liver Total Lipids and Percent Distribution in Lipid Classes
of Acetate-%
Total Lipid (dpm/g)
tomized and ureteral ligation groups, compared to the 48-hr sham group. Incorporation of acetate-14C into the total lipids of spleen, testes, aorta, kidney, and epididymal adipose tissues are shown in Table 8. There were no significant differences in incorporation into any of these tissues between the various groups.
Free Cholesterol (%I
Cholesterol Esters 1%)
Triglycerides (%I
Free Fatty Acods 1%)
Phospholipids (%)
14,075
k 1182
13.4 + 1.0
2.7 r 0.2
15.8 t 1.1
6.2 k 0.9
63.1
+ 2.3
Nephrectomy
17,871
+ 1807
19.0 Yk 1.0
3.5 k 0.3
10.3 * 1.3
6.6 + 0.7
58.9
+ 3.3
Ureteral ligation
14,628
r 544
17.5 t 1.8
3.8 zk 0.2
10.0 + 1.2
7.0 + 1.1
61.3
+ 4.1
48-hr Sham
10,924
+ 470
21.9
t 2.6
3.2 + 0.3
2.0 + 0.4
66.2
? 2.6
Nephrectomy
15,880
k 1368.
36.2
+ 2.9*
2.2 + 0.2
18.3 +_ 1.9*
1.5 * 0.3
42.8
+ 2.8*
Ureteral ligation
13,662
k 775*
47.2
k 2.5’
2.0 f 0.1
13.3 k 1.5*
1.5 * 0.2
36.0
+ 2.1.
*Indicates incorporation into the 48-hr groups, p < 0.0 1.
8.0 f
1.2
nephrectomy and ureteral ligation groups was significantly different from the 48-hr sham
315
UREMIA AND LIPID METABOLISM
Table 7. Specific Radioactivities
Group
Free
Esterified
Cholesterol
Cholesterol
of Individual Liver Lipids
TG
FFA
Phosphollpids
0.5-hr Sham
3310
t 440
196 k 20
1192
+ 179
1175 f 355
1137
?45
Nephrectomy
3272
+ 346
14Bt
1340
+ 191
2205
2 485
1520
+ 106
Ureteral ligation
2272
? 454
161 i 9
1855 k 280
1290
k 90
Sham
2722
? 408
108 k 12
955 k 155
1022
t 30
Nephrectomy
5875
+ 551’
116 + 6
1029 + 134
1085
t 240
964 t 57
Ureteral legation
8687
+ 1032*
95 i 7
1060 + 170
1380 2 235
754 f 45
11
1292 t 181
48-hr 867 + 121
Abbreviabons: TG, triglycerides; FFA, free fatty acids. Values are dpm/mg lipid + SE. *indicates free cholesterol specific activity in the 48-hr nephrectomy and ureteral ligation groups significantly dtfferent from the 48-hr sham.pi0.01.
the 48-hr uremic groups, as has been previously observed in acutely uremic dogsI and in chronically uremic ratsI and humans.’ Unlike uremic humans, but similar to rats uremic for a IO-wk period,” plasma cholesterol concentrations were also increased in the present 48-hr uremic rats. Previous studies of the mechanism of the hypertriglyceridemia in uremic rats have indicated that there is no increase in hepatic triglyceride secretion rate,14.” acetyl CoA carboxylase activity,15 or heparin elutable tissue lipoprotein lipase activity,15 but that a substance present in the plasma of uremic rats may inhibit adipose tissue lipoprotein lipase activity,” and thereby result in a reduced triglyceride clearance rate. A similar inhibitor of lipoprotein lipase activity has been noted in uremic human plasma.16 In the present experiments, plasma triglyceride concentrations and total incorporation of acetate into plasma triglycerides were increased, but specific activities of plasma triglycerides were not increased in the severe uremic groups. In addition, plasma free fatty acids and the proportion of 14C-acetate found in the plasma free fatty acid fraction were lower in the 48-hr uremic groups than in the Table 8.
Incorporation
controls. These results, therefore, suggest that both increased synthesis and a decreased rate of removal may contribute to the hypertriglyceridemia in this 48-hr uremic rat model. Plasma cholesterol concentrations and specific radioactivities were both increased, suggesting a net increased cholesterol synthesis. In vitro studies have shown a twofold increase in sterol synthesis in uremic rat livers, compared to normal.17 Our previous studies in dogs undergoing hemodialysis also suggested a potentiation of cholesterol synthesis from acetate by uremia.” It has been reported that 50%-60% of the metabolism of mevalonate by pathways not leading to cholesterol occurs in the kidneys.“.” Nephrectomy results in decreased CO? production from mevalonate and increased synthesis of liver and plasma cholesterol from mevalonate.‘” It seems possible that the present group with surgical or functional nephrectomies had a decreased capacity to metabolize circulating mevalonate by the shunt pathway, resulting in greater utilization by the liver for cholesterol synthesis, as evidenced by the increased specific activities of liver free cholesterol in these groups. It is likely
of Acetate-‘?
Into Tissue Total Lipids Epldldymal
Group
Spleen
Testes
Aorta
Kidney
Adxpose
0.5-hr Sham
5122
k 293
1403 + 127
3352
+ 125
Nephrectomy
4135
+ 440
1546 f 72
3399
r 991
Ureteral ligation
4813
2 228
1389 2 35
3882
t 2666
9752
7484
6543
f 253
3029
r 347
4115
k 396
k 980
3636
+ 464
? 1264
4533
t 471
3288
+ 292
2983
+ 180
48.hr Sham
4549
+ 228
1253 k 108
3497
+ 653
Nephrectomy
4414
k 320
1735
3781
k 764
Ureteral ligation
5544
t 309
1412 _t 76
2796
+ 762
Values are dpm/g tissue + SE.
+ 102
9897
2 1021
MORIN,
316
therefore that hypercholesterolemia in experimental rat uremia develops by mechanisms dissimilar to the hypertriglyceridemia. Acetate conversion to lipids is altered by uremia, but the mechanisms may not be similar to those in human renal disease patients, since hypercholesterolemia is not usually observed in the latThis may be related to the much longer ter. 2’m23
SRIKANTAIAH.
AND
DAVIDSON
time periods that the investigated human patients were uremic compared to the rat model in the present study. ACKNOWLEDGMENT The authors acknowledge the expert technical assistance Bassist, S. Franklin, J. Ripley, P. Shuss, C. Kimm, D. Wright, and M. Merritt.
of L.
REFERENCES 1. Bagdade JD: Uremic lipemia: An unrecognized abnormality in triglyceride production and removal. Arch Intern Med 126875-881, 1970 2. Nitzan M: Abnormalities of carbohydrate and lipid metabolism in experimentally induced acute uremia. Nutr Metab 15:187-191, 1973 3. Lowrie EG, Lazarus JM, Hampers CL, et al: Survival of patients undergoing chronic hemodialysis and renal transplantation. N Engl J Med 288:864-867, 1973 4. Bagdade JD: Atherosclerosis in patients undergoing maintenance hemodialysis. Kidney Int 7:S370-S372, 1975 5. McCosh EJ, Solangi K, Rivers JM, et al: Hypertriglyceridemia in patients with chronic renal insufficiency. Am J Clin Nutr 28:1036-1043. 1975 6. Novello A, Kelsch R, Easterling RE: Acetate intolerance during hemodialysis. Trans Am Sot Nephrol:66, 1974 7. Gonzales FM, Pearson JE, Barbus SB, et al: On the effects of acetate during hemodialysis. Trans Am Sot Artif InternOrgans 20~169-174, 1974 8. Davidson WD, Moore TD, Glassock RJ, et al: Instantaneous and continuous measurement of “C-labeled substrate oxidation to “C0, by human surgical biopsy specimens: An ionization chamber method. Metabolism 18:10261032.1969 9. Kraml M: A semi-automated determination of phospholipids. Clin Chim Acta 13:442-448, 1966 10. Soloni FG: Simplified manual micromethod for determination of serum triglycerides. Clin Chem 17:529-534, 1971 11. Allain CC, Poon LS, Chan CSG. et al: Enzymatic determination 475,1974 12. Novak determination 1965
of total serum cholesterol.
Clin Chem 20:470-
MJ: Calorimetric ultramicro of free fatty acids. J Lipid
method for the Res 6:431-433,
13. Markeixicz K, Walasek L, Trznadel K, et al: Changes in serum lipid concentrations in acute experimental uremia. Acta Med Pol 15:89-95. 1974 14. Gregg R, Mondon CE, Reaven EP, et al: Effect of acute uremia on triglyceride kinetics in the rat. Metabolism 25:1557-1565, 1976 15. Bagdade JD, Yee E, Wilson DE, et al: Hyperlipidemia in renal failure: Studies of plasma lipoproteins, hepatic triglyceride production, and tissue lipoprotein lipase in a chronically uremic rat model. J Lab Clin Med 91:176186, 1978 16. Murase T, Cattran DC, Rubenstein B, et al: Inhibition of lipoprotein lipase by uremic plasma, a possible cause of hypertriglyceridemia. Metabolism 24: 1279-l 286, 1975 17. Lowenstein LM, Lowenstein JM, Brunengraber H. et al: Lipid abnormalities and atherogenesis in chronic renal failure. Proceedings Ninth Annual Contractor’s Conference, Artificial Kidney Program, NIAMDD, 1976, p 16 18. Morin RJ, Guo LSS, Rorke SJ, et al: Lipid metabolism in non-uremic and uremic dogs during and after hemodialysis with acetate. J Dialysis 2:113-l 29, 1978 19. Edmond J, Fogelman AM, Popjak G: Mevalonate metabolism: Role of kidneys. Science 193:154-156, 1976 20. Wiley MH, Howton MM, Siperstein MD: The quantitative role of the kidneys in the in vivo metabolism of mevalonate. J Biol Chem 252:548-554. 1977 21. Bagdade JD, Porte D Jr, Bierman EL: Hypertriglyceridemia: A metabolic consequence of chronic renal failure. N Engl J Med 269:181-185, 1968 22. Kleinknecht D, Laudat MH, Strauch G, et al: Lipoprotein and carbohydrate disorders in nephrotic syndrome and uremia. Rev Eur Etudes Clin Biol 17:27-3 1, 1972 23. Brons M, Christensen NC. Horder M: Hyperlipoprotein in patients with chronic renal failure. Acta Med Stand 192:119-125,1972
J. Morin,
Mayasandra
U
REMIA results in a hyperlipidemic state in man and animals’,2 and may be a major cause of the increased atherosclerosis and its complications observed in chronic renal disease patients.3’4 The hyperlipidemias and atherosclerosis have been reported in some studies to be worse in renal disease patients undergoing hemodialysis than in those not receiving this treatmenL4” Acetate is the most common alkalinizing agent used during hemodialysis, and these patients are subjected to large unphysiologic plasma acetate loads.6S7 Acetate is a well known lipid precursor, which might contribute to the elevated plasma lipids in these patients. The present investigation was aimed at determining whether experimental uremia alters either the catabolism of acetate to CO, or its conversion to plasma and tissue lipids, so as to gain further insight into the possible aggravating factors in uremic hyperlipidemia. AND
METHODS
Sixty male Sprague-Dawley rats weighing about 200 g were used in this study, and were divided into six groups containing IO rats each. The groups were: (1) sham operated-studied 0.5 hr after operation; (2) bilateral nephrecMetsbolism,
Vol.
29,
No.
4
(April),
1980
Into Rat Plasma
Lipids
V. Srikantaiah.
Experimental uremia was induced in rats by means of bilateral nephrectomy or bilateral ureteral ligation. Incorporation of acetate-l -‘k into expired ‘*CO2 and into plasma and tissue lipids was studied immediately after surgery and at 48 hr, when the rats were uremic. In rats studied immediately after surgery, bilateral nephrectomy. but not bilateral ureteral ligation. significantly decreased the conversion of acetate-l-‘? into expired ‘%O,. In uremic rats at 48 hr. acetate-l -‘% metabolism to “CO, was not significantly altered in either group. Plasma triglyceride concentrations and ‘%-acetate incorporation into triglycerides were increased in the 48-hr uremic groups, but plasma and liver triglyceride specific radioactivities were not significantly altered. Plasma free fatty acid concentrations and incorporation of acetate into free fatty acids were lower in the 48-hr uremic groups than in controls. Plasma cholesterol concentrations and specific radioactivities were increased in these uremic groups, as were liver free cholesterol specific activities. These results suggest that increased triglyceride and cholesterol synthesis from acetate may contribute to the hypertriglyceridemia and hypercholesterolemia observed in uremic rats.
MATERIALS
of Acetate and Warren
D. Davidson
tomy (renal artery ligation)-studied 0.5 hr after ligation: (3) bilateral ureteral ligation-studied 0.5 hr after ligation; (4) sham operated-studied 48 hr after operation; (5) bilateral nephrectomy-studied 48 hr after nephrectomy; and (6) bilateral ureteral ligation-studied 48 hr after ligation. The rats were maintained in the fasting state and then were given acetate-l-‘% (59.0 mCi/mmol. New England Nuclear. Boston, Mass.), 100 &i/kg and nonradioactive acetate, 10 mmole/kg intraperitoneally. “C0Z in expired air from each rat was monitored continuously for 4 hr using a vibrating reed electrometer-ionization chamber method.’ The rats were killed by exsanguination and blood and tissues were obtained for lipid analysis. Total lipids in rat plasma, liver, epididymal adipose tissue, aorta, spleen. testes, and kidney were extracted by homogenization twice in 10 times their volume of chloroform/ methanol, 2/ 1. using a Polytron homogenizer. The combined extracts were washed with acetate buffer (pH 4.0) to remove nonlipid components. Mean recovery of total lipids was 94%. Phospholipid concentrations were determined following digestion of aliquots of the washed lipid extracts at 180°C for 2.5 hr with perchloric acid. Calorimetric phosphate analysis was done by addition of hydrazine sulfate. stannous chloride. and sodium molybdate, and optical densities at 815 nm recorded automatically using a Technicon Autoanalyzcr.’ Plasma triglycerides were extracted into N-nonane and isopropanol (2:3.5, volume:volume). After transesterification with ethoxide, free glycerol was recovered in the aqueous phase and color developed with acetylacetone.‘” The absorbance was read at 410 nm in a Hitachi spectrophotometer. Total plasma cholesterol was determined enzymatically.” In this method, serum cholesterol esters were hydrolyzed to free cholesterol by cholesterol ester hydrolase. The free cholesterol was then oxidized by cholesterol oxidase to cholest4-en-3-one, with the simultaneous production of hydrogen peroxide; the latter oxidatively couples with 4-amino antipyrine and phenol in the presence of peroxidase to yield a chromogen with maximum absorption at 500 nm A single aqueous reagent obtained from Abbott Laboratories. Chicago, Illinois was utilized, and after a IO-min incubation, optical densities were recorded automatically using an Abbott Bichromatic analyzer. Plasma free cholesterol was determined by the same method except that addition of _ From the Departments of Pathology and Medicine, Harbor General Hospital, UCLA School o/ Medicine. Torrance, Calif. Received for publication May 7. 1979. Supported by Artificial Kidney Program (NIH) Contract NOI-AM-S-2209 and NIH Training Grant AM-05383. Address reprint requests to Dr. Robert J. Morin, Department of Pathology. Harbor General Hospital, UCLA School of Medicine, 1000 West Carson Street, Torrance. Calif. 90509. 0 I980 by Grune & Stratton, Inc. 0026-0495/80/2904~003$01.00/0
311
312
MORIN.
SRIKANTAIAH,
AND DAVIDSON
cholesterol ester hydrolase was omitted. Plasma free fatty acids were determined calorimetrically after reaction of cobalt soaps of the free fatty acids with LYnitroso$ naphthol.” For determinations of radioactivities, plasma and liver lipid classes were separated by thin-layer chromatography on silica gel G plates coated with fluorescein. The plates were developed with petroleum ether-diethyl ether-acetic acid (SO:ZO: I), the lipid zones detected under UV light, collected, eluted, and radioactivities in aliquots of these eluates determined by lipid scintillation counting. Mean recovery of lipids was 90.5%. Significance of apparent differences between groups was determined by the t test for unpaired groups. RESULTS
The blood urea nitrogen levels in each of the experimental groups were as follows: sham (OShr), 24.6 mg/dl i 6.7 (SD); bilateral nephrectomy (0.5-hr), 52.9 f 11.6; bilateral ureteral ligation (0.5hr), 38.3 + 9.3; sham (48 hr), 20.8 + 3.8; bilateral nephrectomy (48 hr), 216.5 + 37.6; bilateral ureteral ligation (48 hr), 259.2 + 44.8. The time courses of oxidation of the administered 14C-acetate to “C0, in each of the experimental groups are indicated in Figs. 1 and 2. Percentages of the administered acetate catabolized to CO, over the 4-hr experimental period are shown in Table 1. In rats studied immediately after surgery (mild uremic groups), bilat-
MINUTES Fig. 2. Recovery of “CO, in expired air following intraperitoneal injection of acetate-l-? into uremic rats 48 hr after bilateral ureteral ligation (O---O) or bilateral nephrectomy (O---O) compared to sham operated. nonuremic controls (O---O). Each curve is the mean expired “CO, in 10 rats. The areas under the three curves (total recovery of “COJ are not significantly different.
era1 nephrectomy, but not bilateral ureteral ligation, significantly reduced the recovery of r4C0, from injected acetate-l-14C, compared with sham-operated controls. In the severely uremic rats, neither bilateral nephrectomy nor bilateral ureteral ligation significantly altered recovery of 14C0, from injected acetate- 1-14C, compared with sham operated or mild uremic controls. Results of rat plasma lipid analysis are indicated in Table 2. Free and esterified cholesterol and triglyceride concentrations were significantly elevated in the 4%hr nephrectomized and
ureteral ligation groups, whereas free fatty acids were decreased below the sham-operated controls in both these groups (p < 0.01 for all). As Table 1. “C0,
Recovery After
Acetate-l-‘?
Administration
ii Group
”
I%)
SD I%)
P
0.5-hr 0
30
60
90
120
I60
240
MINUTES Fig. 1. Recoveryof ‘*COz in expired air following intraperitoneal injection of acetate-l -‘*C into nonuremic rats 0.5 hr after bilateral ureteral ligation (O---O), bilateral nephrectomy (O--O), or sham operation (O--O). Each curve represents the mean expired ‘%ZO, in 10 rats. The area under the curve (i.e., recovery) for rats with bilateral nephrectomy is significantly less than in the sham operated rats. *Indicates p > 0.05 (see Table 1).
Sham
10
67.6
5.1
-
Bilateral nephrectomy
10
58.3
6.1
<0.0025*
Bilateral ureteral ligation
10
69.6 8.9
Sham
10
65.1
8.4
-
Bilateral nephrectomy
10
70.7
a.7
>o.o5t
Bilateral ureteral ligation
10
70.5
5.9
>o.o5t
>0.30’
48-hl
*Versus acute shams. tVersus chronic shams.
UREMIA
AND
LIPID
METABOLISM
313
Table 2. Plasma Lipid Concentrations
Group
in Control, Bilateral Nephrectomized.
Free
Esterified
Cholesterol
Cholesterol
and Bilateral Ureteral
TG
Ligated Rats
FFA
Phospholiplds
0.5hr
Sham
22.3
zk 1.1
49.3
2
1.9
25.8
+ 5.5
22.5
I
2.1
118.8
+ 6.1
Nephrectomy
20.7
r
1.5
51.6
f
2.6
24.4
+ 3.2
18.7
c
1.9
102.6
+ 7.0
Ureteral
27.9
+
1.7
52.2
+ 3.1
19.3
+ 2.0
22.3
+
1.3
90.0
5 6.7
Sham
25.6
k 0.8
57.9
+ 3.6
19.6
-i- 1.4
19.9
+
1.9
102.0
k 7.6
Nephrectomy
36.1
k 2.9’
75.1
t
5.5.
59.1
+ 7.2’
14.6
t
1.6*
137.6
+ 7.9
Ureteral
39.3
f
98.4
+ 7.2
50.1
r
15.0
t
2.0
109.0
i
ligation
48-hr
ligation
Abbreviations: Values
TG, triglycerides:
are mg/dl
*Indicates
48-hr
plasma
FFA,
3.0 free fatty
6.2
9.9
acids.
? SE.
nephrectomy
group
significantly
different
from
48-hr
sham,
seen in Table 3, acetate-14C incorporation into rat plasma total lipids was significantly increased in both the 48-hr nephrectomized and ureteral ligation groups compared with the 48-hr sham-operated group (p < 0.01). The percentage of total acetate-14C incorporated into free cholesterol, cholesterol esters, and triglycerides of the former two groups was increased, whereas the percentage incorporated into free fatty acids and phospholipids was decreased below that of Table 3. Incorporation
of Acetate-‘?
Total lbpid Group
p < 0.01
the 48-hr sham group (p < 0.01 for all). Similar results are seen when incorporation of acetate14C was calculated in terms of dpm incorporated into each of the individual plasma lipids/ml plasma. When calculated as specific radioactivity (Table 4, dpm/mg of each lipid class), only plasma free and esterified cholesterol showed an increased incorporation in the 48-hr nephrectomized and ureteral ligation groups compared with the 48-hr sham group (p < 0.01).
Into Plasma Total Lipids and Percent Distribution Free
Cholesterol
Cholesterol
Esters
1%)
(%I
(dpmlml)
in Lipid Classes
Free Fatty Tnglycerldes 1%)
Aads
Phospholipads
1%)
(%l
0.5-hr Sham
1084
k 59
9.2
k 0.6
20.8
k 0.9
27.8
+
1.4
3.3
i
0.2
40.3
1
Nephrectomy
1486
+
125
8.3
k 0.6
20.5
+
1.4
24.0
k 2.3
2.7
-r 0.2
44.2
+ 2.0
Ureteral
1025
f
64
9.9
*
24.8
t
1.4
20.2
+
1.4
2.9
i
0.4
42.6
i
2.5
ligation
0.5
1.6
2.2
48-hr Sham
i- 44
11.9
+ 0.9
23.5
f
13.3
k
1.1
2.9
+ 0.4
44.3
- 3.5
Nephrectomy
1943
739
+
153’
20.5
f
1.6*
37.4
+ 2.9s
22.5
+ 2.3’
1.0
f O.lf
20.5
-
1.8’
Ureteral
ligation
2225
-i
178’
21.3
+
1.7’
40.7
k 2.6*
24.4
k 3.1’
0.9
t
16.4
r
1.2’
that
nephrectomy
*Indicates
the 48-hr
and ureteral
Table 4.
Gr0Ul
ligation
groups
Specific Radioactivities
FrlX
Esterified
Cholesterol
Cholesterol
were
significantly
different
from
0.1
the 48-hr
l
sham
group.
p
I 0.01
of Individual Plasma Lipids
TG
FFA
Phosoholnds
0.5-hr Sham
494
+ 38
338
k 29
1145
-r 229
128
k
15
306
r
18
Nephrectomy
635
2 69
355
+ 38
1535
k 230
204
i
22
550
t
49
Ureteral
398
k 30
283
+ 17
1181
+
110
121
*
10
462
t
37
+ 22
ligation
48-hr Sham
38
189
+ 25
748
f
39
117
f
14
321
Nephrectomy
1184
341
-r 133*
659
+ 106’
752
t
90
121
*
14
325
i
Ureteral
1291
k
543+51*
913
*
109
110
+ 25
325
k 29
ligation
Abbreviations: Values
TG,
are dpm/mg
*Indicates
that
triglycerides: lipid
the 48-hr
FFA,
f
167* free fatty
22
acids.
+ SE. nephrectomy
and ureteral
ligation
groups
were
significantly
different
from
the 48-hr
sham
group.
p J_ 0.01.
314
MORIN,
Table 5. Liver Lipid Concentrations Free Cholesterol
GrOWI
in Control, Nephrectomized, Esterified Cholesterol
SRIKANTAIAH,
and Ureter-Ligated
TG
AND
DAVIDSON
Rats
Phospholipids
FFA
0.5hr Sham
0.8 k 0.05
1.8 r 0.12
7.8 r 0.8
1.02 + 0.42
31.0?
Nephrectomy
1.1 + 0.04
2.1 + 0.12
5.4 + 0.3
1.18 r 0.29
31.1
k 0.6
Ureteral ligation
1.1 + 0.08
1.9 ? 0.09
4.8 k 0.5
0.97
31.8
k 1.2
48-hr Sham
‘_ 0.09
0.8
0.9 + 0.03
2.0 + 0.18
4.5 f 0.5
0.47
c 0.05
30.0
i 0.7
Nephrectomy
0.8 f 0.04
1.8 f 0.10
10.5 + 1.5’
0.46
k 0.04
31.4
+ 0.6
Ureteral ligation
0.8 + 0.06
1.7 f 0.09
6.7 t 0.8
0.34
r 0.04
28.3
+ 0.8
Abbreviations: TG, triglycerides; FFA. free fatty acids. Values are mg/g wet wt liver f SE. *indicates that liver triglyceride concentration was significantly higher in the 48-hr nephrectomy group than in the 48-hr sham group, p < 0.01.
Liver lipid concentrations in these rat groups are given in Table 5. The only significant difference observed was an increase in triglyceride concentration in the 48-hr nephrectomized group compared with the 48-hr sham group (p < 0.01). Incorporation of acetate-i4C into liver total lipids (Table 6) was increased in the 48-hr nephrectomized and ureteral ligation groups compared with the 48-hr sham group (p < 0.01). The percentage of total acetate-14C activity incorporated into free cholesterol and triglycerides of the former two groups was increased, and the phospholipid fraction showed a decreased percentage of incorporation (p < 0.01 for both). Similar results were seen when incorporation was calculated as dpm in each lipid class/g liver, with the exception that incorporation into the phospholipids of the 48-hr nephrectomized group was not significantly different from the 48-hr sham group. As seen in Table 7, when calculated as dpm/mg lipid, only free cholesterol specific activity was higher in the 48-hr nephrecTable 6. Incorporation
Group 0.5hr Sham
DISCUSSION
The present results indicate that severe uremia in rats does not significantly alter the catabolism of acetate to C02, and that the observed differences in incorporation of acetate into plasma and tissue lipids are probably not attributable to differences in availability of substrate between the severe uremic and the control groups. Acetate pool size could not be measured, however, and our conclusions are based upon the assumption that these pool sizes remained the same in the groups compared. Plasma triglyceride levels were increased in
Into Liver Total Lipids and Percent Distribution in Lipid Classes
of Acetate-%
Total Lipid (dpm/g)
tomized and ureteral ligation groups, compared to the 48-hr sham group. Incorporation of acetate-14C into the total lipids of spleen, testes, aorta, kidney, and epididymal adipose tissues are shown in Table 8. There were no significant differences in incorporation into any of these tissues between the various groups.
Free Cholesterol (%I
Cholesterol Esters 1%)
Triglycerides (%I
Free Fatty Acods 1%)
Phospholipids (%)
14,075
k 1182
13.4 + 1.0
2.7 r 0.2
15.8 t 1.1
6.2 k 0.9
63.1
+ 2.3
Nephrectomy
17,871
+ 1807
19.0 Yk 1.0
3.5 k 0.3
10.3 * 1.3
6.6 + 0.7
58.9
+ 3.3
Ureteral ligation
14,628
r 544
17.5 t 1.8
3.8 zk 0.2
10.0 + 1.2
7.0 + 1.1
61.3
+ 4.1
48-hr Sham
10,924
+ 470
21.9
t 2.6
3.2 + 0.3
2.0 + 0.4
66.2
? 2.6
Nephrectomy
15,880
k 1368.
36.2
+ 2.9*
2.2 + 0.2
18.3 +_ 1.9*
1.5 * 0.3
42.8
+ 2.8*
Ureteral ligation
13,662
k 775*
47.2
k 2.5’
2.0 f 0.1
13.3 k 1.5*
1.5 * 0.2
36.0
+ 2.1.
*Indicates incorporation into the 48-hr groups, p < 0.0 1.
8.0 f
1.2
nephrectomy and ureteral ligation groups was significantly different from the 48-hr sham
315
UREMIA AND LIPID METABOLISM
Table 7. Specific Radioactivities
Group
Free
Esterified
Cholesterol
Cholesterol
of Individual Liver Lipids
TG
FFA
Phosphollpids
0.5-hr Sham
3310
t 440
196 k 20
1192
+ 179
1175 f 355
1137
?45
Nephrectomy
3272
+ 346
14Bt
1340
+ 191
2205
2 485
1520
+ 106
Ureteral ligation
2272
? 454
161 i 9
1855 k 280
1290
k 90
Sham
2722
? 408
108 k 12
955 k 155
1022
t 30
Nephrectomy
5875
+ 551’
116 + 6
1029 + 134
1085
t 240
964 t 57
Ureteral legation
8687
+ 1032*
95 i 7
1060 + 170
1380 2 235
754 f 45
11
1292 t 181
48-hr 867 + 121
Abbreviabons: TG, triglycerides; FFA, free fatty acids. Values are dpm/mg lipid + SE. *indicates free cholesterol specific activity in the 48-hr nephrectomy and ureteral ligation groups significantly dtfferent from the 48-hr sham.pi0.01.
the 48-hr uremic groups, as has been previously observed in acutely uremic dogsI and in chronically uremic ratsI and humans.’ Unlike uremic humans, but similar to rats uremic for a IO-wk period,” plasma cholesterol concentrations were also increased in the present 48-hr uremic rats. Previous studies of the mechanism of the hypertriglyceridemia in uremic rats have indicated that there is no increase in hepatic triglyceride secretion rate,14.” acetyl CoA carboxylase activity,15 or heparin elutable tissue lipoprotein lipase activity,15 but that a substance present in the plasma of uremic rats may inhibit adipose tissue lipoprotein lipase activity,” and thereby result in a reduced triglyceride clearance rate. A similar inhibitor of lipoprotein lipase activity has been noted in uremic human plasma.16 In the present experiments, plasma triglyceride concentrations and total incorporation of acetate into plasma triglycerides were increased, but specific activities of plasma triglycerides were not increased in the severe uremic groups. In addition, plasma free fatty acids and the proportion of 14C-acetate found in the plasma free fatty acid fraction were lower in the 48-hr uremic groups than in the Table 8.
Incorporation
controls. These results, therefore, suggest that both increased synthesis and a decreased rate of removal may contribute to the hypertriglyceridemia in this 48-hr uremic rat model. Plasma cholesterol concentrations and specific radioactivities were both increased, suggesting a net increased cholesterol synthesis. In vitro studies have shown a twofold increase in sterol synthesis in uremic rat livers, compared to normal.17 Our previous studies in dogs undergoing hemodialysis also suggested a potentiation of cholesterol synthesis from acetate by uremia.” It has been reported that 50%-60% of the metabolism of mevalonate by pathways not leading to cholesterol occurs in the kidneys.“.” Nephrectomy results in decreased CO? production from mevalonate and increased synthesis of liver and plasma cholesterol from mevalonate.‘” It seems possible that the present group with surgical or functional nephrectomies had a decreased capacity to metabolize circulating mevalonate by the shunt pathway, resulting in greater utilization by the liver for cholesterol synthesis, as evidenced by the increased specific activities of liver free cholesterol in these groups. It is likely
of Acetate-‘?
Into Tissue Total Lipids Epldldymal
Group
Spleen
Testes
Aorta
Kidney
Adxpose
0.5-hr Sham
5122
k 293
1403 + 127
3352
+ 125
Nephrectomy
4135
+ 440
1546 f 72
3399
r 991
Ureteral ligation
4813
2 228
1389 2 35
3882
t 2666
9752
7484
6543
f 253
3029
r 347
4115
k 396
k 980
3636
+ 464
? 1264
4533
t 471
3288
+ 292
2983
+ 180
48.hr Sham
4549
+ 228
1253 k 108
3497
+ 653
Nephrectomy
4414
k 320
1735
3781
k 764
Ureteral ligation
5544
t 309
1412 _t 76
2796
+ 762
Values are dpm/g tissue + SE.
+ 102
9897
2 1021
MORIN,
316
therefore that hypercholesterolemia in experimental rat uremia develops by mechanisms dissimilar to the hypertriglyceridemia. Acetate conversion to lipids is altered by uremia, but the mechanisms may not be similar to those in human renal disease patients, since hypercholesterolemia is not usually observed in the latThis may be related to the much longer ter. 2’m23
SRIKANTAIAH.
AND
DAVIDSON
time periods that the investigated human patients were uremic compared to the rat model in the present study. ACKNOWLEDGMENT The authors acknowledge the expert technical assistance Bassist, S. Franklin, J. Ripley, P. Shuss, C. Kimm, D. Wright, and M. Merritt.
of L.
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13. Markeixicz K, Walasek L, Trznadel K, et al: Changes in serum lipid concentrations in acute experimental uremia. Acta Med Pol 15:89-95. 1974 14. Gregg R, Mondon CE, Reaven EP, et al: Effect of acute uremia on triglyceride kinetics in the rat. Metabolism 25:1557-1565, 1976 15. Bagdade JD, Yee E, Wilson DE, et al: Hyperlipidemia in renal failure: Studies of plasma lipoproteins, hepatic triglyceride production, and tissue lipoprotein lipase in a chronically uremic rat model. J Lab Clin Med 91:176186, 1978 16. Murase T, Cattran DC, Rubenstein B, et al: Inhibition of lipoprotein lipase by uremic plasma, a possible cause of hypertriglyceridemia. Metabolism 24: 1279-l 286, 1975 17. Lowenstein LM, Lowenstein JM, Brunengraber H. et al: Lipid abnormalities and atherogenesis in chronic renal failure. Proceedings Ninth Annual Contractor’s Conference, Artificial Kidney Program, NIAMDD, 1976, p 16 18. Morin RJ, Guo LSS, Rorke SJ, et al: Lipid metabolism in non-uremic and uremic dogs during and after hemodialysis with acetate. J Dialysis 2:113-l 29, 1978 19. Edmond J, Fogelman AM, Popjak G: Mevalonate metabolism: Role of kidneys. Science 193:154-156, 1976 20. Wiley MH, Howton MM, Siperstein MD: The quantitative role of the kidneys in the in vivo metabolism of mevalonate. J Biol Chem 252:548-554. 1977 21. Bagdade JD, Porte D Jr, Bierman EL: Hypertriglyceridemia: A metabolic consequence of chronic renal failure. N Engl J Med 269:181-185, 1968 22. Kleinknecht D, Laudat MH, Strauch G, et al: Lipoprotein and carbohydrate disorders in nephrotic syndrome and uremia. Rev Eur Etudes Clin Biol 17:27-3 1, 1972 23. Brons M, Christensen NC. Horder M: Hyperlipoprotein in patients with chronic renal failure. Acta Med Stand 192:119-125,1972