Metabolism of very long chain polyunsaturated fatty acids in isolated rat germ cells

Which cell type is responsible for the high levels of very long chain polyunsaturated fatty acids in testis and whether this fatty acid pattern is a result of a local synthesis are not presently known. In this study, fatty acid conversion from 20∶4n−6 to 22∶5n−6 and from 20∶5n−3 to 22∶6n−3 was investigated in isolated rat germ cells incubated with [1‐ 14 C]‐labeled fatty acids. The germ cells elongated the fatty acids from 20‐ to 22‐carbon atoms and from 22‐ to 24‐carbon atoms but had a low Δ6 desaturation activity. Thus, little [ 14 C]22∶5n−6 and [ 14 C]22∶6n−3 were synthesized. When Sertoli cells were incubated with [1‐ 14 C]20∶5n−3 for 24 h, an active fatty acid elongation and desaturation were observed. In vivo germ cells normally have a higher content of 22∶5n−6 or 22∶6n−3 than Sertoli cells. An eventual transport of essential fatty acids from Sertoli cells to germ cells was thus studied. Different co‐culture systems were used in which germ cells were on one side of a filter and Sertoli cells on the opposite side. When isolated pachytene spermatocytes or round spermatids were added to the opposite side of a semipermeable filter, approximately 1 nmol [ 14 C]‐22∶6n−3 crossed the filter. Little of this was esterified in the germ cells. Similarly, in using [1‐ 14 C]20∶4n−6 in identical experiments, very little [ 14 C]22∶5n−6 was esterified in germ cells on the opposite side of the filter. Although the very active synthesis of 22∶5n−6 and 22∶6n−3 observed in Sertoli cells suggests a transport of these compounds to germ cells, this was not experimentally determined.