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Enzyme
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Query: EC:3.1.1.79 (
hormone-sensitive lipase
)
2,163
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
By catalyzing the rate-limiting step in adipose tissue lipolysis,
hormone-sensitive lipase
(
HSL
) is an important regulator of energy homeostasis. The role and importance of
HSL
in tissues other than adipose are poorly understood. We report here the cloning and expression of a testicular isoform, designated HSLtes. Due to an addition of amino acids at the NH2-termini, rat and human HSLtes consist of 1068 and 1076 amino acids, respectively, compared to the 768 and 775 amino acids, respectively, of the adipocyte isoform (HSLadi). A novel exon of 1.2 kb, encoding the human testis-specific amino acids, was isolated and mapped to the
HSL
gene, 16 kb upstream of the exons encoding HSLadi. The transcribed mRNA of 3.9 kb was specifically expressed in testis. No significant similarity with other known proteins was found for the testis-specific sequence. The amino acid composition differs from the HSLadi sequence, with a notable hydrophilic character and a high content of prolines and glutamines. COS cells, transfected by the 3.9-kb human testis cDNA, expressed a protein of the expected molecular mass (M(r) approximately 120,000) that exhibited catalytic activity similar to that of HSLadi. Immunocytochemistry localized
HSL
to elongating spermatids and
spermatozoa
;
HSL
was not detected in interstitial cells.
...
PMID:Molecular cloning, genomic organization, and expression of a testicular isoform of hormone-sensitive lipase. 881 77
The present work reports on testicular
hormone-sensitive lipase
(
HSL
), the biological significance of which has been documented in male fertility. The
HSL
protein levels and enzymatic activity were measured, respectively, by densitometry of immunoreactive bands in Western blots, performed with antibodies against recombinant rat
HSL
, and by spectrophotometry in seminiferous tubules (STf) and interstitial tissue (ITf) enriched fractions generated from neonatal, pubertal, and adult guinea pig testes. In addition,
HSL
was studied in subcellular fractions obtained from STf isolated from adult testes and in epididymal
spermatozoa
(Spz). A 104-kDa
HSL
protein was detected in STf and ITf, the expression and activity of which increased with testicular development. Three immunoreactive bands of 104, 110, and 120 kDa were detected in the lysosomal subfraction, and two bands of 104 and 120 kDa were detected in Spz. The
HSL
activity was positively correlated with free (FC) and esterified (EC) cholesterol ratios in STf and ITf, but not with triglyceride (TG) levels, during testicular development. Immunolabeling localized
HSL
to elongated spermatids and Sertoli cells, where its distribution was stage-dependent, and within the cells lining the excurrent ducts of the testis. The findings of the 104- and 120-kDa
HSL
immunoreactive bands and of
HSL
activity in Spz as well, as the detection of the 104-, 110-, and 120-kDa immunoreactive bands in lysosomes, suggest that part of
HSL
may originate from germ cells and be imported in Sertoli cells. The
HSL
protein levels and enzymatic activity in ITf and STf were positively correlated with serum testosterone levels during development. To the best of our knowledge, this study is the first to contribute insights regarding the impact of
HSL
on FC:EC cholesterol ratios and TG levels in the interstitial tissue and tubules in relation to serum testosterone levels during postnatal development, and regarding the immunolocalization of the enzyme in regions of the male gamete consistent with
spermatozoa
-oocyte interaction.
...
PMID:Expression, activity, and subcellular localization of testicular hormone-sensitive lipase during postnatal development in the guinea pig. 1146 32
The 84-kDa
hormone-sensitive lipase
(gene designation Lipe; EC 3.1.1.3) is a cholesterol esterase and triglyceride hydrolase that functions in the release of fatty acids from adipocytes. The role of
hormone-sensitive lipase
in other tissues such as the testis, where a specific 120-kDa testis-specific isoform is expressed, is unknown. To study this, we examined the fertility and testicular histology of gene-targeted
hormone-sensitive lipase
-deficient mice. Homozygous
hormone-sensitive lipase
-deficient male mice are infertile and have decreased testis weights; female homozygotes are fertile. Testicular abnormalities, detected at the light and electron microscopic levels, included the presence of multinucleated round and elongating spermatids, vacuolization of the seminiferous epithelium, asynchronization of the spermatogenic cycle, sloughing of postmeiotic germ cells from the seminiferous epithelium into the lumen, and a marked reduction in the numbers of late spermatids. Extensive nuclear head deformation was noted in late spermatids as well as the sharing of a common acrosome in multinucleated cells. In some multinucleated cells, nuclei were separated from their acrosomes, with the acrosomes remaining attached to areas of ectoplasmic specializations, suggesting defects in intercellular cytoplasmic bridge integrity. Although the lumen of the epididymis was essentially devoid of
spermatozoa
and filled instead with spherical degenerating cells, the epididymal epithelial cells appeared normal. The few late spermatids present in the epididymis were abnormal. There was no morphological evidence, as judged by the absence of lipid droplets of triacylglycerol or cholesteryl ester accumulation in the testis. Together, the data suggest that
hormone-sensitive lipase
deficiency results in abnormalities in spermiogenesis that are incompatible with normal fertility. We speculate that a metabolite downstream from the
hormone-sensitive lipase
reaction may be essential for membrane stabilization and integrity in the seminiferous epithelium and, in particular, may play an important role in the maintenance of intercellular cytoplasmic bridges between postmeiotic germ cells.
...
PMID:Infertility and testicular defects in hormone-sensitive lipase-deficient mice. 1156 84
The role of cholesterol differs in the two compartments of the testis. In the interstitial tissue, cholesterol is necessary for the synthesis of testosterone, whereas in the seminiferous tubules, membrane cholesterol content in developing germ cells will influence the gametes' fertility. Here we evaluate the
hormone-sensitive lipase
(
HSL
) modulation of the cholesterol metabolism in each compartment of the testis. Two
HSL
immunoreactive bands of 104- and 108-kDa were detected in Western blots performed with polyclonal anti-human
HSL
antibodies in the interstitial tissue (ITf)- and seminiferous tubule (STf)-enriched fractions generated from testes harvested at 30-day intervals during puberty and, in the adult mink, during the annual seasonal reproductive cycle. Epididymal
spermatozoa
expressed a 104-kDa
HSL
isoform, and
HSL
was active in these cells. Immunolabeling localized
HSL
to interstitial macrophages; Sertoli cells, where its distribution was stage specific; spermatids; and the equatorial segment of
spermatozoa
. Total
HSL
protein levels, specific enzymatic activity, and free cholesterol (FC):esterified cholesterol (EC) ratios varied concomitantly in STf and ITf and reached maximal values in the adult during the period of maximal spermatogenic activity. In STf,
HSL
-specific activity correlated with FC:EC ratios but not with triglyceride levels. In STf, high
HSL
-specific activity occurred concomitantly with high FSH serum levels. In ITf,
HSL
-specific activity was high during periods of low serum prolactin levels and high serum testosterone levels. The results suggest that 1) modulation of cholesterol metabolism in individual testicular compartments may be regulated by
HSL
isoforms expressed by distinct cells; 2) interstitial macrophages may be part of a system involved in the synthesis of steroid hormones and in the recycling of sterols in the interstitium, whereas in the tubules, recycling could be ensured by Sertoli cells; 3) there is distinctive substrate preference for testicular
HSL
; and 4)
HSL
may be the only cholesterol esterase in this location.
...
PMID:Relationship of the hormone-sensitive lipase-mediated modulation of cholesterol metabolism in individual compartments of the testis to serum pituitary hormone and testosterone concentrations in a seasonal breeder, the mink (Mustela vison). 1260 19
Inactivation of the
hormone-sensitive lipase
gene (HSL) confers male sterility with a major defect in spermatogenesis. Several forms of HSL are expressed in testis. HSLtes mRNA and protein are found in early and elongated spermatids, respectively. The other forms are expressed in diploid germ cells and interstitial cells of the testis. To determine whether the absence of the testis-specific form of HSL, HSLtes, was responsible for the infertility in HSL-null mice, we generated transgenic mice expressing HSLtes under the control of its own promoter. The transgenic animals were crossed with HSL-null mice to produce mice deficient in HSL in nongonadal tissues but expressing HSLtes in haploid germ cells. Cholesteryl ester hydrolase activity was almost completely blunted in HSL-deficient testis. Mice with one allele of the transgene showed an increase in enzymatic activity and a small elevation in the production of
spermatozoa
. The few fertile hemizygous male mice produced litters of very small to small size. The presence of the two alleles led to a doubling in cholesteryl ester hydrolase activity, which represented 25% of the wild type values associated with a qualitatively normal spermatogenesis and a partial restoration of sperm reserves. The fertility of these mice was totally restored with normal litter sizes. In line with the importance of the esterase activity, HSLtes transgene expression reversed the cholesteryl ester accumulation observed in HSL-null mice. Therefore, expression of HSLtes and cognate cholesteryl ester hydrolase activity leads to a rescue of the infertility observed in HSL-deficient male mice.
...
PMID:The testicular form of hormone-sensitive lipase HSLtes confers rescue of male infertility in HSL-deficient mice. 1529 23
Hormone-sensitive lipase (
HSL
, Lipe, E.C.3.1.1.3) is a multifunctional fatty acyl esterase that is essential for male fertility and spermatogenesis and that also plays important roles in the function of adipocytes, pancreatic beta-cells, and adrenal cortical cells. Gene-targeted
HSL
-deficient (
HSL
-/-) male mice are infertile, have a 2-fold reduction in testicular mass, a 2-fold elevation of the ratio of esterified to free cholesterol in testis, and unique morphological abnormalities in round and elongating spermatids. Postmeiotic germ cells in the testis express a specific
HSL
isoform. We created transgenic mice expressing a normal human testicular
HSL
cDNA from the mouse protamine-1 promoter, which mediates expression specifically in postmeiotic germ cells. Testicular cholesteryl esterase activity was undetectable in
HSL
-/- mice, but in
HSL
-/- males expressing the testicular transgene, activity was 2-fold greater than normal.
HSL
transgene mRNA became detectable in testes between 19 and 25 days of age, coinciding with the first wave of postmeiotic transcription in round spermatids. In contrast to nontransgenic
HSL
-/- mice,
HSL
-/- males expressing the testicular transgene were normal with respect to fertility, testicular mass, testicular esterified/free cholesterol ratio, and testicular histology. Their cauda epididymides contained abundant, normal-appearing
spermatozoa
. We conclude that human testicular
HSL
is functional in mouse testis and that the mechanism of infertility in
HSL
-deficient males is cell autonomous and resides in postmeiotic germ cells, because
HSL
expression in these cells is in itself sufficient to restore normal fertility.
...
PMID:Expression of human hormone-sensitive lipase (HSL) in postmeiotic germ cells confers normal fertility to HSL-deficient mice. 1534 79
In male mice, deficiency of hormone sensitive lipase (
HSL
, Lipe gene, E.C.3.1.1.3) causes deficient spermatogenesis, azoospermia, and infertility. Postmeiotic germ cells express a specific
HSL
isoform that includes a 313 amino acid N-terminus encoded by a testis-specific exon (exon T1). The remainder of testicular
HSL
is identical to adipocyte
HSL
. The amino acid sequence of the testis-specific exon is poorly conserved, showing only a 46% amino acid identity with orthologous human and rat sequences, compared with 87% over the remainder of the
HSL
coding sequence, providing no evidence in favor of a vital functional role for the testis-specific N-terminus of
HSL
. However, exon T1 is important for Lipe transcription; in mouse testicular mRNA, we identified 3 major Lipe transcription start sites, finding numerous testicular transcription factor binding motifs upstream of the transcription start site. We directly explored two possible mechanisms for the infertility of
HSL
-deficient mice, using mice that expressed mutant
HSL
transgenes only in postmeiotic germ cells on a
HSL
-deficient background. One transgene expressed human
HSL
lacking enzyme activity but containing the testis-specific N-terminus (
HSL
-/-muttg mice). The other transgene expressed catalytically inactive
HSL
with the testis-specific N-terminal peptide (
HSL
-/-atg mice).
HSL
-/-muttg mice were infertile, with abnormal histology of the seminiferous epithelium and absence of
spermatozoa
in the epididymal lumen. In contrast,
HSL
-/-atg mice had normal fertility and normal testicular morphology. In conclusion, whereas the catalytic function of
HSL
is necessary for spermatogenesis in mice, the presence of the N-terminal testis-specific fragment is not essential.
...
PMID:The catalytic function of hormone-sensitive lipase is essential for fertility in male mice. 2479 31
