Dietary Protein and the Blood Glucose Concentration

نویسندگان

  • Frank Q. Nuttall
  • Mary C. Gannon
چکیده

Body proteins are being synthesized and degraded continuously (1). The estimated turnover is w210 g/day (2). Amino acids resulting from protein degradation can be recycled (reused for synthesis), but this is incomplete. Therefore, dietary protein is necessary for maintenance of lean body mass. Also, dietary protein is required to replace protein lost from the shedding of skin, hair, nails, cells in the gastrointestinal tract, and protein-containing secretions. However, the actual losses are estimated to be only 6–8 g/day (3). Overall, approximately w32–46 g of high-quality dietary protein/day is reported to be required to maintain protein balance (2). This is considerably less than amounts of protein reportedly consumed by American adults (w65– 100+ g/day) (4). The excess food-derived amino acids then are oxidized as fuel directly or indirectly after conversion to glucose. In 1915, using a phlorhizinized dog preparation, Janney (5) demonstrated clearly that the deaminated amino acids (carbon skeletons) present in dietary proteins could be used to produce glucose endogenously. For most common proteins, 50–80 g of glucose can be derived from 100 g of ingested protein. Nevertheless, as early as 1913, Jacobson (6) reported that ingestion of proteins did not raise the blood glucose. Later, in 1924, MacLean (7) fed 50 g of meat protein to two subjects, one with and one without mild diabetes. The theoretical amount of glucose that could be produced was 25 g. However, there was no change in blood glucose. He then fed the subjects 25 g glucose and the blood glucose was clearly elevated. In 1936, Conn and Newburgh (8) reported that ingestion of even a very large amount of protein as meat (1.3 pounds, 0.59 kg), did not raise the blood glucose. Subsequently, the degradation pathways for each amino acid were elucidated. Of the 20 amino acids found in proteins, all but leucine could, at least in part, be converted into glucose and thus contribute to the circulating glucose pool. However, data from many laboratories, including our own, confirmed that ingested protein per se does not increase the circulating glucose concentration (9,10). The reason for this remained unknown. In order to address this issue, a number of years ago (11) we determined the actual amount of glucose entering the circulating glucose pool using a glucose isotope-dilution technique. Urea formation was determined as an index of the amount of ingested protein deaminated, and the carbon skeletons available for glucose synthesis. Normal, young subjects ingested 50 g of cottage cheese protein (casein). It was calculated that 34 g were deaminated (68%) over the 8 h of the study. The amount of glucose produced and entering the circulation was only 9.7 g (11). Thus, the amount of glucose produced was considerably less than the amount theorized (w25 g). The plasma glucose concentration did not change. Later, in people with untreated type 2 diabetes, ingestion of 50 g beef protein was calculated to result in only 2.0 g of additional glucose added to the circulation over the 8-h study period (12). These results were rather surprising because, as expected, the basal glucose production rate in the diabetic subjects was greater than that in normal young subjects (13–15). Interestingly, numerous studies now have demonstrated that provision of any of the commonly ingested gluconeogenic substrates, fructose, galactose, glycerol, as well as amino acids, when infused or ingested do not, or only modestly, increase hepatic production and release of glucose (16) and have little effect on the circulating glucose concentration. This is due to a hepatic autoregulatory process which is independent of a change in the circulating insulin or glucagon concentrations (17,18). In this issue of Diabetes, Fromentin et al. (19) have elegantly addressed the issue of the endogenous partitioning of the absorbed amino acids derived from a food (egg) protein. They specifically address the disposition of the carbon skeletons derived from the total amino acids and the appearance rate and quantity of glucose entering the plasma pool over an 8-h period using multitracer technology. Their study is unique in four ways: First, whole eggs were used as a source of protein, i.e., a modest amount of fat as well as protein was ingested. Second, the amount of protein ingested (23 g) was lower than others had used and is well within an amount likely to be ingested in a single meal. Third, diet-derived carbon and nitrogen stableisotope tracers were used. Thus, both the fate of the amino moiety as well as the amino acid carbon chains were traced. This labeling was accomplished by adding doubly labeled amino acids to the diet of laying hens. Fourth, subjects were encouraged to ingest a defined diet containing 14% protein for 5 days prior to the study. The authors calculated that w18 g (79%) of the 23 g of ingested protein could be accounted for by deamination; thus those carbon skeletons were available for gluconeogenesis and release of new glucose into the circulation. The remainder, presumably, was used for new protein synthesis. The total amount of glucose entering the circulation from all sources was calculated to be 50 g over the 8-h period. However, only 4 g (8%) could be attributed to the ingested protein. This was less than a theoretical maximum, From the Endocrinology, Metabolism and Nutrition Section, Minneapolis VA Health Care System, Minneapolis, Minnesota; the Department of Medicine, University of Minnesota, Minneapolis, Minnesota; and the Department of Food Science and Nutrition, University of Minnesota, St. Paul, Minnesota. Corresponding author: Frank Q. Nuttall, [email protected]. DOI: 10.2337/db12-1829 2013 by the American Diabetes Association. Readers may use this article as long as the work is properly cited, the use is educational and not for profit, and the work is not altered. See http://creativecommons.org/licenses/by -nc-nd/3.0/ for details. See accompanying original article, p. 1435.

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عنوان ژورنال:

دوره 62  شماره 

صفحات  -

تاریخ انتشار 2013